EP0070159A2 - Centrifuging apparatus and methods for separating fluids into components thereof - Google Patents

Centrifuging apparatus and methods for separating fluids into components thereof Download PDF

Info

Publication number
EP0070159A2
EP0070159A2 EP82303594A EP82303594A EP0070159A2 EP 0070159 A2 EP0070159 A2 EP 0070159A2 EP 82303594 A EP82303594 A EP 82303594A EP 82303594 A EP82303594 A EP 82303594A EP 0070159 A2 EP0070159 A2 EP 0070159A2
Authority
EP
European Patent Office
Prior art keywords
bag
blood
component
container
flow
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Granted
Application number
EP82303594A
Other languages
German (de)
French (fr)
Other versions
EP0070159A3 (en
EP0070159B1 (en
Inventor
Allen Latham, Jr.
Donald W. Schoendorfer
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
Haemonetics Corp
Original Assignee
Haemonetics Corp
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Priority claimed from US06/281,655 external-priority patent/US4421503A/en
Priority claimed from US06/281,649 external-priority patent/US4402680A/en
Application filed by Haemonetics Corp filed Critical Haemonetics Corp
Priority to AT82303594T priority Critical patent/ATE31033T1/en
Publication of EP0070159A2 publication Critical patent/EP0070159A2/en
Publication of EP0070159A3 publication Critical patent/EP0070159A3/en
Application granted granted Critical
Publication of EP0070159B1 publication Critical patent/EP0070159B1/en
Expired legal-status Critical Current

Links

Images

Classifications

    • BPERFORMING OPERATIONS; TRANSPORTING
    • B04CENTRIFUGAL APPARATUS OR MACHINES FOR CARRYING-OUT PHYSICAL OR CHEMICAL PROCESSES
    • B04BCENTRIFUGES
    • B04B5/00Other centrifuges
    • B04B5/04Radial chamber apparatus for separating predominantly liquid mixtures, e.g. butyrometers
    • B04B5/0407Radial chamber apparatus for separating predominantly liquid mixtures, e.g. butyrometers for liquids contained in receptacles
    • B04B5/0428Radial chamber apparatus for separating predominantly liquid mixtures, e.g. butyrometers for liquids contained in receptacles with flexible receptacles
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B04CENTRIFUGAL APPARATUS OR MACHINES FOR CARRYING-OUT PHYSICAL OR CHEMICAL PROCESSES
    • B04BCENTRIFUGES
    • B04B13/00Control arrangements specially designed for centrifuges; Programme control of centrifuges

Definitions

  • the present invention relates to centrifuging apparatus and methods for separating fluids into components thereof.
  • Applicants' Application No. 80300198.1 describes a centrifuge (hereinafter the Latham centrifuge) for separating one or more components of blood into precise fractions.
  • Such centrifuges operate under the principle that fluid components having different densities or sedimentary rates may be separated in accordance with such densities or sedimentary rates by subjecting the fluid to a centrifugal field.
  • a flexible, disposable blood processing bag is mounted within the rotor of a self-balancing centrifuge rotor in a contoured/pro- cessing chamber consisting of a pair of support shoes.
  • the contoured chamber is designed to support the blood bag in a position whereby separated blood components traverse a short distance in the process of separation.
  • a flexible displacer bag is employed as a movable diaphragm to apply pressure to the disposable blood bag in response to the introduction of displacement fluid into the displacer bag while the centrifuge rotor is either rotating or stationary. Such pressure tends to expel separated blood components from the disposable blood bag.
  • the flexible blood processing and displacer bags are located radially outward from a centrally located collection chamber.
  • a pressure of 7977.04 N/mm 2 must be generated by the displacer fluid to expel blood compoents from the processing bag into the collection chamber.
  • this force can amount to 14768 N and the generation of such large forces tends to move or push the contoured shoes apart.
  • the requirement for a contoured shoe limits the volume of the blood processing bag to a size that will fit into the contours of the shoe.
  • the cost of fabricating the bags should be kept to a minimum.
  • the bags must not rupture under the tremendous forces they are subjected to during the centrifuge process. If these forces are minimized, the bags can be constructed of low-cost materials.
  • a need therefore exists for a blood processing centrifuge apparatus which is capable of handling different volumes of whole blood, does not require a supply of displacer fluid, minimizes the pressure to which the blood processing bags are subjected and provides for automatic termination of flow once a desired quantity of components has been expelled.
  • the present invention provides, from one aspect, apparatus for use in the centrifugal separation of blood into at least a first blood component and a second blood component comprising: a flexible blood processing bag for containing anti-coagulated whole blood and having an outlet port; a receiver container for receiving a component of said whole blood and having an input port; and tubing means providing fluid communication between the output port of the bag and the input port of the receiver container; characterised by valve means for terminating flow of fluid component out the output port of the bag in response to the specific gravity of said component.
  • the present invention further provides apparatus for processing fluids in a centrifugal force field to separate constituent components of such fluids comprising in combination: a centrifuge having a rotor adapted to rotate at a sufficient speed to cause said components to separate; a flexible bag for containing a first fluid; and a receiver container for receiving at least one component of said first fluid; characterised by mass means disposed nearer the center of rotation of the rotor than the flexible bag and adapted to move and contact a surface of said bag, said mass being sufficient to at least initiate a flow from said bag to said container of component fluid separated in said bag.
  • the present invention still further provides a method in which blood is centrifugally separated into a first blood component and second blood component in a-blood processing chamber and first blood component is thereafter caused to flow through an outlet port of said chamber through a conduit and into a receiver container; characterised by causing said flow by a weight disposed adjacent said chamber.
  • the present invention is particularly useful for various pheresis processes such as plasma pheresis or platelet-pheresis.
  • the apparatus of the present invention may comprise a centrifuge of the type described in our concurrently filed Application No.
  • the flexible bag containing the whole blood is located on the rotor a suitable distance away from the center of rotation of the rotor.
  • the receiver container is disposed adjacent the bag and in fluid communication with the bag.
  • the receiver container is adapted to receive one or more of the centrifugally separated components of the whole blood.
  • the receiver container is shown as a flexible bag, however, it need not be. flexible.
  • a pressure plate in the form of a body of material, such as a metal plate, having a predetermined mass is slideably disposed in the radial direction between the flexible bag and the center of rotation of the rotor.
  • This pressure plate is suspended so that it is free to move radially against the flexible bag when subjected to the centrifugal forces generated by rotation of the centrifuge.
  • the pressure plate has a predetermined mass sufficient to-at least initiate a flow of separated fluid component from the flexible bag to the second bag as the pressure plate presses against the first bag during rotation of the centrifuge.
  • the pressure plate has a predetermined mass distribution and shape adapted to pool the separated first blood component in the area of the output of the fluid communication to the second bag.
  • the pressure plate is adapted to press against the first bag and cause the radius at the output of the first bag to be located at the minimum radius of the first bag in the centrifuge.
  • a suitable timing mechanism such as that described in Applicants' concurrently filed Application No. , is provided for controlling the flow of components from the first to the second bag until sufficient separation has been achieved.
  • the first bag and second bag are located adjacent each other on the rotor with the first bag positioned radially inward from the second bag.
  • a siphon effect is created when flow is initiated from the first bag to the second bag due to the difference in centrifugal forces to which the bags are subjected because one bag is located nearer the center of rotation than the other.
  • flow from the first bag to the second bag, once initiated will continue regardless of the specific gravity of the separated blood component.
  • a valve is provided.
  • Pheresis Valve may be in the form of a stopper having a specific gravity less than the component or components to be retained in the first bag, but greater than the component or components to be expressed into the second bag.
  • the stopper may be a free-floating ball, a ball contained within guide channels or a flap attached at one end to an interior surface of the blood processing bag adjacent to its outlet port, or other similar stoppers.
  • the stopper is provided in a disposable software set designed for use in a Self-Balancing Centrifuge.
  • the software consists of a flexible blood-processing bag having an inlet port and an outlet port and being suitable for mounting in the processing chamber of a Self-Balancing Centrifuge.
  • Blood compatible tubing extends between the inlet port of the blood-processing bag and a connector to a source of blood to be separated.
  • a source of blood might be a human donor, in which case the connection means might be a phlebotomy needle, or the source may be a bag containing whole blood, in which case the connection means might be a bag spike.
  • the disposable software also includes a receiver container for first blood component which is expelled from the processing bag.
  • the receiver container is connected to the outlet port of the flexible blood-processing bag so that expelled first blood component can be directed into the receiver container.
  • the flexible blood-processing bag also contains valve means for sealing its outlet port in response to the difference between the specific gravities of separated first and second blood components.
  • An example of a suitable means for sealing is a valve with a stopper which has a specific gravity which is higher than the specific gravity of first blood component but lower than the specific gravity of second blood component.
  • the stopper may be a free-floating ball, a ball contained within guide channels, a flap attached at one end to an interior surface of the blood-processing bag adjacent to its outlet port, or other similar stoppers.
  • the valve operates in a fully automatic way depending only on the difference in specific gravities between the separated components.
  • the valve is versatile in the sense that it can be adapted to provide a precise cut between any number of different blood components based upon their specific gravity difference.
  • the precise cut can also be adjusted by changing the.size of the stopper, e.g., providing a large or small diameter ball, or by changing its shape.
  • the use of such a stopper eliminates the extreme precision required in the geometry and weight of a pressure plate if a precise cut in blood components is to be made.
  • the stopper can be made an intergral part of the software supplied for use in any particular blood separation.
  • valve may be made intentionally leaky so that the stopper is unseated and additional separation may be made by re-cycling the valve.
  • first and second bags are disposed adjacent each other substantially equidistant from the center of rotation of the rotor.
  • the mass of the pressure plate positioned against the first bag is such that it is.of sufficient value to create just enough force against the first bag to express only the less dense component(s) from the first bag to the second bag.
  • the second bag is located closer to the center of rotation than the first bag and the mass of the weight plate is such that it produces sufficient pressure to express specific lighter components of blood in the second bag but lacks sufficient pressure to express specific heavier components from the first bag.
  • a low-cost aseptic, disposable apparatus in combination with a centrifuge system wherein blood components may be automatically separated from whole blood without the need for displacer fluid or contoured shoes.
  • An apparatus of the invention is able to accomodate various volumes of whole blood for processing and may be operated by unskilled personnel since human intervention is minimized.
  • the present invention includes an apparatus and method for separating blood into components thereof in a centrifuge.
  • the invention is particularly suitable for various pheresis processes, such as, (a) plasma-pheresis, where in whole blood is removed from a donor, separated into cell-free plasma and packed red blood cells followed by re- infusion of the autologous red cells or (b) platelet-pheresis, wherein whole blood is removed from a donor and separated into three components, platelet-rich plasma (PRP), platelet-poor plasma (PPP) and packed red blood cells (RBC) followed by reuniting the PPP and RBC which are returned to the donor, or similar component separation where the donor donates a unit of blood which is separated into plasma and packed red cells; plasma, platelets and packed red cells; or plasma, platelets, white cells and packed red cells.
  • PRP platelet-rich plasma
  • PPP platelet-poor plasma
  • RBC packed red blood cells
  • the invention will generally be described in connection with component separation of whole blood into plasma, platelets, and packed red cells by centrifugal separation in accordance with the specific gravity of the components but the invention is not intended to be limited thereby.
  • separation in accordance with the sedimentation rate of individual components is also contemplated by this invention.
  • FIG. 1 For simplicity, only a top view of the Self-balancing Centrifuge 2 is shown in Fig. 1.
  • the apparatus shown in Fig. 1 is adapted to conduct two pheresis processes simultaneously and therefore has duplicate process apparatus within each half of the rotor of centrifuge 2.
  • Rigid cassettes 17 are mounted on opposite sides of the rotor of centrifuge 2 within cylindrical housing 34.
  • Each cassette 17 consists of a stand, or rack, which is partitioned into three annular sections by two vertically positioned support members 22 and 24 each having a shape generally described by a segment of a hollow cylinder with a radius corresponding to the radius to the center of rotation of the centrifuge rotor (as shown in detail in Fig. 4).
  • a sufficient volume of anticoagulant may be initially stored in the whole blood bag 8 or the appropriate anticoagulant ratio may be pumped with the blood.
  • tube 50 is heat sealed close to bag 8 and the section of tube 50 containing the phlebotomy needle is disconnected and discarded.
  • a pressure plate 10 is suspended adjacent the whole blood bag 8 on two mounting bolts 91 and 93 (shown in Fig. 4)
  • Bag 8 is loaded in the cassette while pressure plate 10 is moved radially inward. This allows sealed bag 8 filled with anticoagulated whole blood to be inserted into the space between the plate 10 and the cassette wall 22.
  • the PRP bag 6 is inserted into the next section of the cassette and the PPP bag 4 in the last section, which is the section furthest removed from the center of rotation.
  • An additional pressure plate 11 may be provided adjacent the side of the PRP bag 6 nearest the center of rotation. As will be described in detail later, this pressure plate cooperates with a flexible elastomeric gasket to isolate platelets and prevent them from flowing out the PPP tube 54.
  • the PRP tubing 52 and PPP tubing 54 are initially clamped "off" by operation of the hydraulic timer mechanism 15.
  • the centrifuge 2 is then brought to a suitable speed, for example, 2000 r.p.m., . for a sufficient time to allow centrifugal separation of PRP and packed RBC's within bag 8, i.e. about one minute.
  • the hydraulic timer 15 then unclamps the PRP tubing 52 by rotating clamp 31.
  • the pressure exerted by the weight plate 10 on the whole blood bag 8 as the rotor continues to spin is sufficient to force the plasma separated in bag 8, which is of lower density, out the exit port of the bag and into PRP tubing 52, which is centrally located on the side of the whole blood bag nearest the center of rotation.
  • the weight plate is needed here as initially the PRP must be pushed toward the center of rotation of the rotor as it leaves the blood bag.
  • the difference in potential energy from the whole blood bag 8 to the PRP bag 6 favors flow in that direction and pressure from the pressure plate 10 is no longer required to maintain flow.
  • the plate still serves a useful function to prevent the buildup of excessive dynamic waves on the inner wall of the blood bag.
  • This siphon effect is advantageous in that the mass of the pressure plate 10 and the pressure that it generates in the centrifugal force field is minimized. Therefore, the pressure holding capacity of the blood bags is greatly reduced and lower cost disposable plastics bags may be utilized. On the other hand, once initiated, fluid flow will continue, therefore, means are required to automatically stop the flow of plasma before any RBC is lost.
  • this automatic flow control means (shown generally at 117) is provided by a Pheresis Valve with a ball stopper 112 having a specific gravity greater than PRP (about 1.03) but less than that of RBC
  • This ball stopper is located in the whole blood bag 8 so as to float on top of the
  • RBC layer 116 A separated first blood component, such as plasma layer 114, occupies the radially inner portion of the flexible blood-processing bag 8 whereas separated second blood component such as RBC layer 116, occupies the radially outward portion.
  • the pressure plate 10 applies a force in the radially outward direction (arrows A) which tends to collapse the flexible blood processing bag 8 and expel first blood component (plasma layer) 114 therefrom.
  • the stopper ball 112 is contained within a guide member 119 formed by a cylindrical wall member 118, an end wall member 120, and a stopper ball seat 122.
  • the cylindrical wall member 118 has one or more input ports 124 located relatively close to the stopper ball seat 122.
  • Separated first blood component (PRP) enters the input port(s) (as shown by arrows B) in the cylindrical wall member 118 and leavesthe flexible blood bag 8 and flows through output port 128 into tubing 52 in the direction of arrow C to PRP bag 6.
  • the inner diameter of the cylindrical wall member 118 is chosen such that the stopper ball is free to move axially within guide 119 in the direction C, but not radially of the wall member 118.
  • the end wall member contains one or more end wall ports 124. When the radial depth of the first blood component 114 is greater than the radial depth of the end wall member 120 within the flexible blood processing bag 8, the stopper ball 112 rides on is supported by, the end wall member.
  • the interface between said first and second components approaches the output port 128, of the flexible whole blood-bag 8.
  • the stopper ball 112 also approaches the output port 128.
  • the stopper ball 112 is carried into contact with the seat of guide 119 and forms a seal with the port. This is illustrated in Fig. 7 wherein substantially all of the first blood component 114 has been expelled from the flexible, whole blood bag 8 and all that remains is second blood component 116.
  • flow is thus immediately halted automatically.
  • the specific gravity of the stopper ball 112 is chosen so that it floats on the interface between the first and second blood components 114 and 116. That is, the stopper ball 112 has a specific gravity greater than the specific gravity of the second blood component 116.
  • the specific gravity of the stopper ball 112 is preferably chosen to be about midway between these values.
  • Typical materials for the.ball stopper is Dow Corning silicone which comes in specific gravities within this range and can be supplied with FDA Class VI certification, or conventional polystyrene.
  • the embodiments thus far described have operated on the principle that the blood component with the greater density, for example RBC, is retained in the container and the less dense component PRP is allowed to flow to another container, in some applications it may be desirable to reverse the process. For example, if the-outlet port and valve seat is located adjacent the more dense component, and a ball float with an intermediate density is disposed to float on the interface, as the more dense component is expressed out the port the interface and ball would move toward the valve seat and close in the manner previously described.
  • the blood component with the greater density for example RBC
  • a simple and inexpensive solution is illustrated.
  • the output port for tubing 52 on whole blood bag 8 is oriented by pressure-plate 10 to be at a minimum radius with respect to the radius of the bag 8 from the center of rotation.
  • any air in the bag 8 will collect in the area of the output port.
  • tubing 52 is unclamped by clamp 31 of mechanism 15, this air must flow out of the bag 8 and into the PRP bag 6 before any plasma will flow.
  • the section of tubing labelled 52B has an unusually small internal diameter, ID 2 as compared to a normal inner diameter ID 1 on the remaininq section 52A of tubing 52.
  • Section 52B is the section of tubing which extends radially outward from the clamp -15 and therefore fluid in this section is in effect forced to flow downhill with the centrifugal force. With the internal diameter reduced in this section, the velocity of flow increases and air bubbles which would otherwise be trapped in this section are forced to flow "down" the tube 52 to PRP bag 6.
  • a similar reduced diameter tubing is not required in tube 54 as there is no need for an umbilical fitment on PRP bag 6 as there was in the whole blood bag 8. Because of this, air in bag 6 is not localized in the area of the output port and therefore is not expressed from bag 6 with the PPP.
  • a barrier 802 is provided intermediate the PPP output port and the PRP input port.
  • This barrier may be conveniently made by conventional heat or R.F. sealing during the fabrication of the bag 6.
  • the barrier should preferably extend along the length of the bag from the input ports to about one inch from the bottom as shown by the vertically extending solid and dotted lines in Fig. 8.
  • Fig. 8 also shows a preferred embodiment of the apparatus for fixing the final volume of the platelet concentrate (PRP) left in PRP bag 6.
  • Pressure plate 11 is free to move radially against PRP bag 6 under the influence of centrifugal force.
  • the plate 11 is of sufficient size to eclipse one side of bag 6.
  • the other side of PRP Bag 6 abuts fixed support member 24.
  • a flexible elastomeric gasket 806 is affixed to support member 24 of cassette 17 in a radial plane.
  • the PRP/PPP separation apparatus functions as follows:
  • PPP tubing 54 is unclamped. As separated PPP flows from the PRP bag 6, the bag tends to collapse and pressure plate 11 approaches the elastomeric gasket 806 and eventually compresses the PRP bag against the gasket forming a transverse barrier along the length of gasket 806 thereby preventing further flow out the PPP tube thus isolating the remaining plasma, which, for the reasons previously given, will be rich in platelets.
  • the location of the elastomeric gasket in relation to the height of the PRP bag 6 and the thickness of the gasket is adapted to isolate a predetermined volume of plasma in the PRP bag 6.
  • a predetermined volume of plasma in the PRP bag 6 For example, in the embodi- . ment of Fig. 8, 50 milliliters can be retained with a 1/16" ID by 1/8" OD tube gasket located one-third down the height of a 6" x 10" bag.
  • pressure plate 11 also functions to prevent formation of dynamic waves on the inner surface of the PRP bag 6.
  • mass of the pressure plate may be varied by adding or subtracting mass and thereby controlling the flow of PRP from the whole blood bag. A more massive pressure plate on the PRP bag in relation to the mass of the pressure plate on the whole blood bag 8 will decrease the rate of PRP flow since it will increase the back pressure on PRP bag 6.
  • Pressure plate 11 may also be fashioned with a section 803 cut out on the side opposite the PPP and PRP tubes 52 and 54.
  • This cut out section 803 allows the PRP bag to bulge out within the cut out section. Since this bulge is pushed radially inward, any air 809 in PRP bag 6 will be pushed into the bulge and be isolated from the PPP output tube 54. This acts as a safety factor to prevent the vapor lock effect from occurring in tube 54.
  • clamps 31 and '35 of timer mechanism 15 clamp PRP tube 52 and PPP tube 54 and the centrifuge rotor is brought to rest.
  • the end result of this process is a bag of packed RBC, a bag of PRP in bag 6 and a bag of PPP in bag 4.
  • Figs. 9 and 10 the effect of the size of the stopper ball 112 on the precise blood cut achieved is illustrated.
  • the ball stopper 112 has a relatively large diameter and tends to contact and seal outlet port 128 prior to the expulsion of all the first blood component l14. If the first blood component 114 is plasma and the second blood component 116 is packed red cells, the effect of the larger diameter ball stopper 112 is to lower the hematocrit of the second blood component remaining in the blood processing bag 8. On the other hand, when a relatively smaller diameter ball stopper is employed, such as in Fig. 10, a much smaller amount of PRP 114 remains in the flexible blood processing bag 8. Thus, the hematocrit of the second blood component or packed red cells 116 is raised.
  • Fig. 11 shows a further embodiment of a Pheresis Valve for sealing the outlet port of a flexible blood processing bags.
  • a hinged flap 110 has one end joined to an interior surface of the flexible blood-processing bag 8 at a position adjacent to the outlet port 128.
  • the hinged flap 110 is of a density similar to that of the stopper ball 112 and operates in a manner . similar to the stopper ball 112 previously described in that it floats at the interface between first blood component 114 and second blood component 116.
  • the hinged flap is carried' into contact with the outlet port 128 thereby creating the required seal.
  • One way to make the valve re-open is to minimize the negative pressure force in the direction C of Fig. 6 and maximize the positive buoyancy force in the opposite direction created by the volume of fluid left in the bag 8. This could be accomplished by decreasing the cross-sectional area of the output tube 52 and increasing the size and therefore the buoyant volume of the valve float. The latter is undesirable since it increases the manufacturing cost of the bag and the former increases the disruptive shear stresses of blood components flowing through the valve, thereby increasing the probability of occlusions.
  • Fig. 12 is a cross-sectional view taken along the lines 12-12 of Fig. 7.
  • the valve seat 122 is made leaky by one or more tiny slots 212 on the valve seat 122 so that the negative downstream pressure is dissipated.
  • the slots leak about 1 millilitre per minute when the ball valve is seated.
  • FIG. 13 and 14 A further embodiment of the invention in which the PRP bag pressure plate 1-1 is eliminated is shown in Figs. 13 and 14.
  • the PRP input port for tubing 52 and output port for PPP tubing 54 are located at the top of PRP bag 6.
  • the timer clamp 15 is located as close to rotor housing 34 as possible.
  • the inner diameter of the PPP tubing 54 is large enough so that the capillary air bubble surface tension inside the tube is less than the centrifugal force'pressure on the fluid in the tube.
  • the PPP tube 54 and bag 4 are empty.
  • the air in the PPP tubing 54 is locked by the plasma.
  • the air surface in the tube 54 cannot withstand the outward pressure of the plasma and this air is displaced out of the PPP tubing 54 into bag 6.
  • a mass clamp 302 such as a 1.27 mm thick strip of plastics, may be disposed adjacent the inner wall of bag 6 opposite the ramp and near the outlet to PPP tubing 54. This mass clamp 302 will terminate PPP flow at a predetermined volume. Such volume may, for example, be at a ratio of 50 ml of plasma for each single unit platelet concentrate left in PRP bag 6 as presently specified by clinical standards.
  • first blood processing bag nearer to the center of rotation than the second bag (which as aforesaid may merely be a rigid receptacle for receiving separated components) as in the embodiments heretofore illustrated, it may be desirable to have a "side-hv-side" arrangement in which the first and second bags are located along the periphery or the rotor housing equidistant to the center of rotation as giagrammatically illustrated in Fig. 15
  • a centrifuge 140 of the type previously described rotates about a center of rotation labelled "CR".
  • the centrifuge rotor housing 142 supports two flexible bags 144 and 146 in a vertical position on the periphery of the rotor and equidistant from the center of rotation.
  • a contoured framework 150 with concave inwardly extending surfaces allows bag 144 to rest naturally against the housing inner surface with a minimum of stress on the bag wall material when subjected to centrifugation. Alignment pins (not shown) keep the bag 144 properly oriented.
  • Inner wall 152 of bag 144 is essen- .tially free-standing except for a light weight, stiff, curved pressure plate 148 disposed against the surface of inner wall 152 so as to produce a liquid pressure in the bag when subjected to the centrifugal field.
  • Interconnecting tubing 154 is provided between the exit port of first bag 144 and the second bag 146 (in this case the receiver container). This tubing passes over a curvilinear contour (or dam) 156 which may be incorporated into the framework 150.
  • This contour is sufficiently large to assure that the exit port of bag 144 is at a lesser distance from the center of rotation than any other portion of the bag 144.
  • the shape of the container is such that the fluid pathway in the first bag near the exit port is in the form of an approach ramp with gradually decreasing radius for locations progressively closer to the exit port.
  • the second bag 146 is merely a receiving container for the separated component from the first bag.
  • the volume of this container is pre-established to just accomodate the volume of separated component (supernatant) desired to be recovered from bag 144.
  • Suitable support means (not shown) hold bag 146 in place against rotor housing 142. Flow from bag 144 to bag 146 is terminated by setting the volume of the second bag 146 so that it is filled completely before all the supernatant has passed from the first bag 144.
  • the pressure in the first bag is proportional to the difference between the squares of the radii to the input and output of the fluid column, to the density of the fluid in the column, and to the square of the rotatinq speed.
  • the density of packed RBC is about 1.10, whereas the density of the supernatant plasma is about 1.03. Greater pressure is therefore required to force red cells radially inward to a given radial point than is required to force plasma at this point. Therefore, when the cut is being made, flow from bag 144 to bag 146 will automatically cease when RBC pass part of the way through the radial passage 154 to the second bag 146, provided the weight of prcs- sure plate 148 is suitably matched to the process.
  • the operating protocol must include a first period of centrifugation while the interconnecting tubing is clamped shut as by the previously described timer mechanism 15 or equivalent. Then the clamp may be opened and clear supernatant may be passed over into the bag in the second compartment 146 until packed RBC flow part way through the interconnecting pathway.
  • Fig. 16 is an improved version of the Fig. 15 apparatus wherein the pressure plate 148 is made large enough in surface area to cover the entire area of wall surface 152 of first blood processing bag 144, thus no bulging is possible. Additionally, the center of gravity of pressure plate 148 is off-centered slightly to a point labelled 164; thereby automatically providing a more optimal separation zone. The center of gravity may be off-set by contouring the shape of plate 148 or by adding or subtracting material from the plate as required. The dam or ramp 156 previously located on the rotor housing is now located on the pressure plate 152 and moves with the plate thereby providing a more constant ramp function.
  • Figs. 15-16 the separation process may be extended in a variety of ways as shown for example in Fig. 17 by adding a pressure plate 180 on bag 146 and interconnecting bag 146 over a second dam 184 to a third bag 182.
  • a process similar to the three bag pheresis process described in connection with Figs. 1-8 may then be carried out by clamping the interconnecting tubing with clamps 185 and 187 at appropriate intervals and centrifugally separating RBC and plasma from whole blood in bag 144.
  • the plasma is then expressed to bag 146 by means of a pressure plate 148 having a mass just sufficient to express the lighter weight plasma sideways over the dam 156 and into bag 146.
  • the plasma in bag 146 is centrifugally separated into PRP and PPP.
  • the PPP is expressed sideways over the second dam 184 by the force of pressure plate 180 which is preestablished so as to express all but a fixed volume of fluid, for example 50 ml, into the fhird bag 182.
  • the clamps 185 and 187 may be controlled by a hydraulic timer mechanism as described earlier.
  • FIG. 18 Another application of the invention' is shown in the embodiment of Fig. 18 which illustrates red blood cell washing apparatus.
  • Fig. 18 three flexible bags 190, 192, and 194 are disposed about the periphery of the rotor housing 142 of centrifuge 140 equidistant from the center of rotation CR.
  • Bag 190 contains a washing solution, such as a solution of sterile saline.
  • Bag 194 is interconnected with bag 190 by tubing 196 and with spent solution bag 192 by tubing 198 which extends over dam 195.
  • Clamp means 191 and 193 operated by a timer mechanism (not shown) control the flow of fluid through respective tubing 196 and 198. :
  • Bag 194 is substantially similar to the blood processing bags previously described. It contains the whole blood or thawed glyceralized blood to be washed.
  • the final product of this procedure is a unit of packed washed red cells.
  • the hematocrit of the packed cells can be made very high.
  • the clamps for this procedure may-be controlled by the hydraulic timer clamp mechanism previously mentioned.
  • Fig. 19 The apparatus described in Fig. 19 is illustrated in connection with the present apparatus, however, the invention described in this embodiment may be applied to a variety of blood processing apparatus and methods.
  • the interconnecting tubing 52 between whole blood bag 8 and PRP bag 6 is shown disposed between a light transmitter element 250 and photo-detector 252 of a well-known beam optical sensor 260.
  • Beam sensor 260 may alternatively comprise a simple reflective optical beam sensor.
  • Tubing 52 also passes between a solenoid activated flow clamp 254.
  • the component line 52 will be clamped. This will trap the RBC's in the whole blood bag 8 and the plasma in the PRP bag 6. Similar apparatus can be used to sense the color change between PPP and PRP to actuate an additional clamp on the tubing 54 between the PRP bag and PPP bag.

Abstract

Centrifuging apparatus 2 has a plate 10 disposed adjacent a flexible whole blood bag 8 in which blood is being processed. Under the influence of centrifugal force the plate 10, which is disposed inwardly nearer the center of rotation than the bag 8, expels a separated blood component from the bag into a receiver bag 6. The bag 6 is located radially outward from the bag 8 and a valve 117 (see Figure 6) is provided which is responsive to the specific density of separated components to stop the flow. The mass of the plate 10 may be selected so as to expel only the desired component. A further separated blood component is similarly expressed into radially outermost bag 4. Timer mechanism 15 automatically clamps the intermediate flow tubing (52, 54). A plurality of embodiments are described useful for plasma pheresis, platelet pheresis and cell-washing.
The receiver bag 6 may be positioned radially inward of bag 8 or circumferentially along side it.
The apparatus minimises the pressure to which blood processing bags are subjected and provides for automatic displacement of separated components and automatic termination of flow within the confines of the rotor.

Description

  • The present invention relates to centrifuging apparatus and methods for separating fluids into components thereof.
  • The desirability and/or necessity of separating whole blood into its components is gaining wide recognition. For example, it has been pointed out that limiting a transfusion to only those blood components necessary for a particular purpose preserves the available supply of blood, and in many situations is better for the patient. Additionally, in many therapeutic techniques, it is necessary to separate one blood component and to reinfuse that component after it has been processed or to substitute the same component from another source.
  • Applicants' Application No. 80300198.1 describes a centrifuge (hereinafter the Latham centrifuge) for separating one or more components of blood into precise fractions. Such centrifuges operate under the principle that fluid components having different densities or sedimentary rates may be separated in accordance with such densities or sedimentary rates by subjecting the fluid to a centrifugal field.
  • In the Latham centrifuge, a flexible, disposable blood processing bag is mounted within the rotor of a self-balancing centrifuge rotor in a contoured/pro- cessing chamber consisting of a pair of support shoes. The contoured chamber is designed to support the blood bag in a position whereby separated blood components traverse a short distance in the process of separation. A flexible displacer bag is employed as a movable diaphragm to apply pressure to the disposable blood bag in response to the introduction of displacement fluid into the displacer bag while the centrifuge rotor is either rotating or stationary. Such pressure tends to expel separated blood components from the disposable blood bag.
  • In a typical embodiment of the Latham centrifuge, the flexible blood processing and displacer bags are located radially outward from a centrally located collection chamber. The pressure required to expel blood components from the processing bag is given by the formula: p = (r0 2 - r1 2) w2 wherein r0 is the radial distance from the center-of rotation to the blood bag and r1 is the radial distance from the center of rotation to the point of collection and w is the rate of rotation. For a 138.43 mm rotor radius and a 50.80 mm collection point radius with the centrifuge rotating at a speed of 2000 r.p.m. and an average blood component density of 1.05 gm/ 3, a pressure of 7977.04 N/mm2 must be generated by the displacer fluid to expel blood compoents from the processing bag into the collection chamber. In a typical application,where the blood processing bag is 152.40 mm by 254.00 mm, this force can amount to 14768 N and the generation of such large forces tends to move or push the contoured shoes apart.
  • It has been proposed by the Applicants to_ provide a weight, or pressure, plate (hereinafter the Schoendorfer pressure plate) adjacent the inner wall of the support shoe nearest the center of rotation of the rotor in the Latham centrifuge. The mass of this pressure plate is chosen to at least equalize the inner pressure generated by the processing bags under the influence of centrifugal force. The pressure plate serves to maintain the contoured shoes securely against the blood processing bags.
  • Nevertheless, while the Latham centrifuge as modified by the Schoendorfer pressure plate operates satisfactorily for the purpose intended, a number of improvements are desirable to make the apparatus less complex, more flexible in application, and lower in cost.
  • For example, the requirement for a contoured shoe limits the volume of the blood processing bag to a size that will fit into the contours of the shoe.
  • Also, the necessity for introducing a displacer fluid creates additional complexity. It becomes necessary to either introduce a displacer fluid from an external source, as in the Latham centrifuge, or to provide a reservoir of displacer fluid on the rotor.
  • Additionally, in order to have blood processing bags which are disposable, the cost of fabricating the bags should be kept to a minimum. On the other hand, the bags must not rupture under the tremendous forces they are subjected to during the centrifuge process. If these forces are minimized, the bags can be constructed of low-cost materials.
  • A need therefore exists for a blood processing centrifuge apparatus which is capable of handling different volumes of whole blood, does not require a supply of displacer fluid and minimizesthe pressure to which the blood processing bags are subjected.
  • Furthermore, the elemination of an external control over the displacement of fluid creates the concomitant problem as to how flow of components from one bag to another may be conveniently terminated at the right moment for establishing prime fractionation.
  • A need therefore exists for a blood processing centrifuge apparatus which is capable of handling different volumes of whole blood, does not require a supply of displacer fluid, minimizes the pressure to which the blood processing bags are subjected and provides for automatic termination of flow once a desired quantity of components has been expelled.
  • The present invention provides, from one aspect, apparatus for use in the centrifugal separation of blood into at least a first blood component and a second blood component comprising: a flexible blood processing bag for containing anti-coagulated whole blood and having an outlet port; a receiver container for receiving a component of said whole blood and having an input port; and tubing means providing fluid communication between the output port of the bag and the input port of the receiver container; characterised by valve means for terminating flow of fluid component out the output port of the bag in response to the specific gravity of said component.
  • The present invention further provides apparatus for processing fluids in a centrifugal force field to separate constituent components of such fluids comprising in combination: a centrifuge having a rotor adapted to rotate at a sufficient speed to cause said components to separate; a flexible bag for containing a first fluid; and a receiver container for receiving at least one component of said first fluid; characterised by mass means disposed nearer the center of rotation of the rotor than the flexible bag and adapted to move and contact a surface of said bag, said mass being sufficient to at least initiate a flow from said bag to said container of component fluid separated in said bag.
  • The present invention still further provides a method in which blood is centrifugally separated into a first blood component and second blood component in a-blood processing chamber and first blood component is thereafter caused to flow through an outlet port of said chamber through a conduit and into a receiver container; characterised by causing said flow by a weight disposed adjacent said chamber.
  • The present invention is particularly useful for various pheresis processes such as plasma pheresis or platelet-pheresis. The apparatus of the present invention may comprise a centrifuge of the type described in our concurrently filed Application No.
  • and hereinafter referred to as a "Self-Balancing Centrifuge". The flexible bag containing the whole blood is located on the rotor a suitable distance away from the center of rotation of the rotor. The receiver container is disposed adjacent the bag and in fluid communication with the bag. The receiver container is adapted to receive one or more of the centrifugally separated components of the whole blood. In the embodiments described below, the receiver container is shown as a flexible bag, however, it need not be. flexible. In these embodiments also, a pressure plate in the form of a body of material, such as a metal plate, having a predetermined mass is slideably disposed in the radial direction between the flexible bag and the center of rotation of the rotor. This pressure plate is suspended so that it is free to move radially against the flexible bag when subjected to the centrifugal forces generated by rotation of the centrifuge. The pressure plate has a predetermined mass sufficient to-at least initiate a flow of separated fluid component from the flexible bag to the second bag as the pressure plate presses against the first bag during rotation of the centrifuge. The pressure plate has a predetermined mass distribution and shape adapted to pool the separated first blood component in the area of the output of the fluid communication to the second bag. The pressure plate is adapted to press against the first bag and cause the radius at the output of the first bag to be located at the minimum radius of the first bag in the centrifuge.
  • A suitable timing mechanism, such as that described in Applicants' concurrently filed Application No. , is provided for controlling the flow of components from the first to the second bag until sufficient separation has been achieved.
  • In one embodiment described below, the first bag and second bag are located adjacent each other on the rotor with the first bag positioned radially inward from the second bag. In this embodiment, a siphon effect is created when flow is initiated from the first bag to the second bag due to the difference in centrifugal forces to which the bags are subjected because one bag is located nearer the center of rotation than the other. Thus, flow from the first bag to the second bag, once initiated, will continue regardless of the specific gravity of the separated blood component. In this erbodi- ment, therefore, a valve is provided. This valve hereinafter called a Pheresis Valve may be in the form of a stopper having a specific gravity less than the component or components to be retained in the first bag, but greater than the component or components to be expressed into the second bag. The stopper may be a free-floating ball, a ball contained within guide channels or a flap attached at one end to an interior surface of the blood processing bag adjacent to its outlet port, or other similar stoppers.
  • In a preferred embodiment, the stopper is provided in a disposable software set designed for use in a Self-Balancing Centrifuge. The software consists of a flexible blood-processing bag having an inlet port and an outlet port and being suitable for mounting in the processing chamber of a Self-Balancing Centrifuge. Blood compatible tubing extends between the inlet port of the blood-processing bag and a connector to a source of blood to be separated. Such a source of blood might be a human donor, in which case the connection means might be a phlebotomy needle, or the source may be a bag containing whole blood, in which case the connection means might be a bag spike.
  • The disposable software also includes a receiver container for first blood component which is expelled from the processing bag. The receiver container is connected to the outlet port of the flexible blood-processing bag so that expelled first blood component can be directed into the receiver container.
  • - The flexible blood-processing bag also contains valve means for sealing its outlet port in response to the difference between the specific gravities of separated first and second blood components. An example of a suitable means for sealing is a valve with a stopper which has a specific gravity which is higher than the specific gravity of first blood component but lower than the specific gravity of second blood component. The stopper may be a free-floating ball, a ball contained within guide channels, a flap attached at one end to an interior surface of the blood-processing bag adjacent to its outlet port, or other similar stoppers.
  • Thus, there is provided a simple but expedient means for accompanying a precise cut between blood components.- The valve operates in a fully automatic way depending only on the difference in specific gravities between the separated components. The valve is versatile in the sense that it can be adapted to provide a precise cut between any number of different blood components based upon their specific gravity difference. Furthermore, the precise cut can also be adjusted by changing the.size of the stopper, e.g., providing a large or small diameter ball, or by changing its shape. Additionally, the use of such a stopper eliminates the extreme precision required in the geometry and weight of a pressure plate if a precise cut in blood components is to be made. Finally, the stopper can be made an intergral part of the software supplied for use in any particular blood separation.
  • Additionally, the valve may be made intentionally leaky so that the stopper is unseated and additional separation may be made by re-cycling the valve.
  • In another embodiment described below, the first and second bags are disposed adjacent each other substantially equidistant from the center of rotation of the rotor. The mass of the pressure plate positioned against the first bag is such that it is.of sufficient value to create just enough force against the first bag to express only the less dense component(s) from the first bag to the second bag.
  • In a third embodiment, the second bag is located closer to the center of rotation than the first bag and the mass of the weight plate is such that it produces sufficient pressure to express specific lighter components of blood in the second bag but lacks sufficient pressure to express specific heavier components from the first bag.
  • Thus, in the various embodiments of the invention, a low-cost aseptic, disposable apparatus is provided in combination with a centrifuge system wherein blood components may be automatically separated from whole blood without the need for displacer fluid or contoured shoes. An apparatus of the invention is able to accomodate various volumes of whole blood for processing and may be operated by unskilled personnel since human intervention is minimized.
  • Specific embodiments of the present invention in all its apparatus and method aspects will now be described in detail by way of example, and not by way of limitation, with reference to drawings in which:
    • Fig. 1 is a top view of centrifuging apparatus in accordance with the present invention.
    • Fig. 2 is a partial side view of a hydraulic timer clamp of the apparatus of Fig. 1 taken along the lines 2-2 of Fig. 1. -
    • Fig. 3 is a perspective of the apparatus in accordance with the present invention for use in the centrifugal separating blood into first, second and third blood components in a centrifuging apparatus of the present invention.
    • Fig. 4 is an enlarged view of part of the apparatus of Fig. 1.
    • Fig. 5 is a partial plan view showing details of the apparatus of Fig. 1.
    • Fig. 6 is a partial cross-section along the lines 6-6 of Fig. 5 showing further details of the apparatus.
    • Fig. 7 is a further cross-sectional detail of the apparatus.
    • Fig. 8 is an enlarged perspective view of a detail of the apparatus taken along the lines 8-8 of Fig. 5.
    • Fig. 8A is a cross-section taken along the lines 8A-8A of Fig. 8.
    • Fig. 9 is a partial cross-section similar to Fig. 6 showing the details of a modification.
    • Fig. 10 is a cross-section similar to Fig. 9 showing the details of a further modification.
    • Fig. 11 is a cross-sectional detail of a still further modification.
    • Fig. 12 is a sectional view taken along lines 12-12 of Fig. 7.
    • Fig. 13 is a partial plan view corresponding to Fig. 5 of a further embodiment of centrifuging apparatus in accordance with the present invention.
    • Fig. 14 is a view of Fig. 13 taken along lines 14-14 of Fig. 13.
    • Fig. 15 is a simplified schematic top view of a further centrifuging apparatus in accordance with the present invention.
    • Fig. 16 is a simplified schematic top sectional view of a still further centrifuging apparatus in accordance with the present invention.
    • Fig. 17 is a simplified top sectionalview of a still further centrifuging apparatus in accordance with the present invention.
    • Fig. 18 is a simplified top sectional view of a still further centrifuging apparatus in accordance with the present invention.
    • Fig. 19 is a schematic diagram of a modification of the centrifuging apparatus in accordance with the present invention.
  • As used herein, the following terms are defined to mean:
    • "First blood component" -- one fraction of blood which it is desired to separate from another fraction;
    • "Second blood component" -- another fraction separated from blood which is the balance after first blood component has been separated therefrom;
    • "Platelet-rich plasma" or "PRP" -- a fraction of plasma which is rich in platelets;
    • "Platelet-poor plasma" or "PPP" -- a fraction of plasma which is poor in platelets;
    • "Packed red blood cells" or "RBC" -- a fraction of blood which is rich in red blood cells.
  • In general, it may be seen that the present invention includes an apparatus and method for separating blood into components thereof in a centrifuge. The invention is particularly suitable for various pheresis processes, such as, (a) plasma-pheresis, where in whole blood is removed from a donor, separated into cell-free plasma and packed red blood cells followed by re- infusion of the autologous red cells or (b) platelet-pheresis, wherein whole blood is removed from a donor and separated into three components, platelet-rich plasma (PRP), platelet-poor plasma (PPP) and packed red blood cells (RBC) followed by reuniting the PPP and RBC which are returned to the donor, or similar component separation where the donor donates a unit of blood which is separated into plasma and packed red cells; plasma, platelets and packed red cells; or plasma, platelets, white cells and packed red cells.
  • For purposes of explanation, the invention will generally be described in connection with component separation of whole blood into plasma, platelets, and packed red cells by centrifugal separation in accordance with the specific gravity of the components but the invention is not intended to be limited thereby. For example, separation in accordance with the sedimentation rate of individual components is also contemplated by this invention
  • In the apparatus of Figs. 1-11, the following main items are illustrated:
    • (1) a Self-Balancing Centrifuge 2 (Fig. 1);
    • (2) a cassette 29 (Fig. 4) for holding sterilized blood processing software 27 (Fig. 3);
    • (3) a cassette software package 27 (Fig. 3) consisting of a whole blood bag 8.containing the correct volume of anticoagulant (CPD-Al), a PRP bag 6 and a PPP bag 4, suitably interconnected by tubing, and a phlebotomy needle 110 connected to the whole blood processing bag 8;
    • (4) a timer mechanism 15 (Fig. 2) such as the Hydraulic Timer Clamp described and shown in the
  • Applicants' concurrently filed Application No.
    • (5) one or more pressure plates 10 (Fig. 4); and
    • (6) a Pheresis Valve 117 (Figs. 9-11) incorporated into the cassette software package.
  • The above-mentioned items and their interrelationship will be described in detail below in connection with the figures.
  • Whilst it is contemplated that a Self-Balancing Centrifuge, or equivalent, will supply the necessary centrifugal force for blood processing and a Pheresis Valve, or equivalent, will provide the means for automatically terminating flow once a precise cut is achieved between components, the invention as described herein is not intended to be limited to the use of such devices.
  • For simplicity, only a top view of the Self-balancing Centrifuge 2 is shown in Fig. 1. The apparatus shown in Fig. 1 is adapted to conduct two pheresis processes simultaneously and therefore has duplicate process apparatus within each half of the rotor of centrifuge 2. Rigid cassettes 17 are mounted on opposite sides of the rotor of centrifuge 2 within cylindrical housing 34.
  • Each cassette 17 consists of a stand, or rack, which is partitioned into three annular sections by two vertically positioned support members 22 and 24 each having a shape generally described by a segment of a hollow cylinder with a radius corresponding to the radius to the center of rotation of the centrifuge rotor (as shown in detail in Fig. 4).
  • A sufficient volume of anticoagulant may be initially stored in the whole blood bag 8 or the appropriate anticoagulant ratio may be pumped with the blood.
  • After the bag 8 is filled with whole blood, tube 50 is heat sealed close to bag 8 and the section of tube 50 containing the phlebotomy needle is disconnected and discarded. A pressure plate 10 is suspended adjacent the whole blood bag 8 on two mounting bolts 91 and 93 (shown in Fig. 4)
  • on the side nearest the center of rotation and in such a manner that the plate 10 is free to move or float against the whole blood bag 8 under the influence of centrifugal force when the rotor is spinning. Bag 8 is loaded in the cassette while pressure plate 10 is moved radially inward. This allows sealed bag 8 filled with anticoagulated whole blood to be inserted into the space between the plate 10 and the cassette wall 22. The PRP bag 6 is inserted into the next section of the cassette and the PPP bag 4 in the last section, which is the section furthest removed from the center of rotation.
  • An additional pressure plate 11 may be provided adjacent the side of the PRP bag 6 nearest the center of rotation. As will be described in detail later, this pressure plate cooperates with a flexible elastomeric gasket to isolate platelets and prevent them from flowing out the PPP tube 54.
  • The respective tubing 52 and 54 interconnecting the PRP bag 6 with the whole blood bag 8 and the PPP bag 4 with the PRP bag 6 are inserted in respective clamps 31 and 35 of the hydraulic timer mechanism 15.
  • In operation, the PRP tubing 52 and PPP tubing 54 are initially clamped "off" by operation of the hydraulic timer mechanism 15. The centrifuge 2 is then brought to a suitable speed, for example, 2000 r.p.m., . for a sufficient time to allow centrifugal separation of PRP and packed RBC's within bag 8, i.e. about one minute. The hydraulic timer 15 then unclamps the PRP tubing 52 by rotating clamp 31.
  • The pressure exerted by the weight plate 10 on the whole blood bag 8 as the rotor continues to spin is sufficient to force the plasma separated in bag 8, which is of lower density, out the exit port of the bag and into PRP tubing 52, which is centrally located on the side of the whole blood bag nearest the center of rotation. The weight plate is needed here as initially the PRP must be pushed toward the center of rotation of the rotor as it leaves the blood bag.
  • Once fluid starts flowing from the whole blood bag 8 to the PRP bag 6 a siphon effect is created, inasmuch as the whole blood bag 8 is located at a shorter radius than the PRP bag and therefore at a higher potential energy.
  • Under these conditions, once the PRP tubing 52 is filled with fluid, the difference in potential energy from the whole blood bag 8 to the PRP bag 6 favors flow in that direction and pressure from the pressure plate 10 is no longer required to maintain flow. However, the plate still serves a useful function to prevent the buildup of excessive dynamic waves on the inner wall of the blood bag.
  • This siphon effect is advantageous in that the mass of the pressure plate 10 and the pressure that it generates in the centrifugal force field is minimized. Therefore, the pressure holding capacity of the blood bags is greatly reduced and lower cost disposable plastics bags may be utilized. On the other hand, once initiated, fluid flow will continue, therefore, means are required to automatically stop the flow of plasma before any RBC is lost.
  • In the preferred embodiment shown in Fig. 6 of the invention, this automatic flow control means (shown generally at 117) is provided by a Pheresis Valve with a ball stopper 112 having a specific gravity greater than PRP (about 1.03) but less than that of RBC
  • (about 1.10). This ball stopper is located in the whole blood bag 8 so as to float on top of the
  • RBC layer 116. A separated first blood component, such as plasma layer 114, occupies the radially inner portion of the flexible blood-processing bag 8 whereas separated second blood component such as RBC layer 116, occupies the radially outward portion. As illustrated, the pressure plate 10 applies a force in the radially outward direction (arrows A) which tends to collapse the flexible blood processing bag 8 and expel first blood component (plasma layer) 114 therefrom.
  • The stopper ball 112 is contained within a guide member 119 formed by a cylindrical wall member 118, an end wall member 120, and a stopper ball seat 122. The cylindrical wall member 118 has one or more input ports 124 located relatively close to the stopper ball seat 122. Separated first blood component (PRP) enters the input port(s) (as shown by arrows B) in the cylindrical wall member 118 and leavesthe flexible blood bag 8 and flows through output port 128 into tubing 52 in the direction of arrow C to PRP bag 6.
  • The inner diameter of the cylindrical wall member 118 is chosen such that the stopper ball is free to move axially within guide 119 in the direction C, but not radially of the wall member 118. The end wall member contains one or more end wall ports 124. When the radial depth of the first blood component 114 is greater than the radial depth of the end wall member 120 within the flexible blood processing bag 8, the stopper ball 112 rides on is supported by, the end wall member.
  • As the first blood component 114 is expressed from the flexible blood processing bag 8 by the force of pressure plate 10 moving in the direction A the interface between said first and second components approaches the output port 128, of the flexible whole blood-bag 8. The stopper ball 112 also approaches the output port 128. Eventually, the stopper ball 112 is carried into contact with the seat of guide 119 and forms a seal with the port. This is illustrated in Fig. 7 wherein substantially all of the first blood component 114 has been expelled from the flexible, whole blood bag 8 and all that remains is second blood component 116. When the stopper ball 112 comes into contact with the outlet port, flow is thus immediately halted automatically.
  • As previously noted, the specific gravity of the stopper ball 112 is chosen so that it floats on the interface between the first and second blood components 114 and 116. That is, the stopper ball 112 has a specific gravity greater than the specific gravity of the second blood component 116. For example, if the first blood component is plasma which has a specific gravity of about 1.03, and the second blood component comprises mostly RBC which has a specific gravity of about 1.10, the specific gravity of the stopper ball 112 is preferably chosen to be about midway between these values. Typical materials for the.ball stopper is Dow Corning silicone which comes in specific gravities within this range and can be supplied with FDA Class VI certification, or conventional polystyrene.
  • While the embodiments thus far described have operated on the principle that the blood component with the greater density, for example RBC, is retained in the container and the less dense component PRP is allowed to flow to another container, in some applications it may be desirable to reverse the process. For example, if the-outlet port and valve seat is located adjacent the more dense component, and a ball float with an intermediate density is disposed to float on the interface, as the more dense component is expressed out the port the interface and ball would move toward the valve seat and close in the manner previously described.
  • It should be noted that it air bubbles accumulate in any sections of the PRP tubing 52 which are extending radially toward the center of rotation (increasing in radius from the whole blood bag 8) a vapor lock may occur in the line. In the embodiment thus far described, the pressure required to initiate the flow of plasma l14 from the whole blood bag 8 to the PRP Bag 6 through tubing 52 is developed by the centrifugal force on pressure plate lυ. Once the flow of plasma nas begun and the PRP tubing 52 is full, the siphon effect previously described dominates the flow. This is one of the advantages of the inner/outer bag geometry of this first embodiment. High flow rates can be reached without the need for a heavy pressure plate 10. On the other hand, if a vapor lock occurs in tube 52, flow will either be diminished or stopped completely. Since the introduction of air in small quantities into the software set is probably unavoidable, a solution to this problem is imperative.
  • In the embodiment shown in Figs. 2 and 5, a simple and inexpensive solution is illustrated. As shown in Fig. 5, the output port for tubing 52 on whole blood bag 8 is oriented by pressure-plate 10 to be at a minimum radius with respect to the radius of the bag 8 from the center of rotation. Thus, any air in the bag 8 will collect in the area of the output port. When tubing 52 is unclamped by clamp 31 of mechanism 15, this air must flow out of the bag 8 and into the PRP bag 6 before any plasma will flow.
  • As indicated in Fig. 5, the section of tubing labelled 52B has an unusually small internal diameter, ID2 as compared to a normal inner diameter ID1 on the remaininq section 52A of tubing 52. Section 52B is the section of tubing which extends radially outward from the clamp -15 and therefore fluid in this section is in effect forced to flow downhill with the centrifugal force. With the internal diameter reduced in this section, the velocity of flow increases and air bubbles which would otherwise be trapped in this section are forced to flow "down" the tube 52 to PRP bag 6. A similar reduced diameter tubing is not required in tube 54 as there is no need for an umbilical fitment on PRP bag 6 as there was in the whole blood bag 8. Because of this, air in bag 6 is not localized in the area of the output port and therefore is not expressed from bag 6 with the PPP.
  • We have thus described how the packed red cells 116 may be separated from the plasma 114 in whole blood bag 8 and the plasma expressed/siphoned over to PRP bag 6 and the flow of the plasma automatically stopped by the Pheresis Valve 117. The details of the process and apparatus for separating platelets from the plasma 114 in PRP bag 6 and expressing the PPP to PPP bag 4 will now be described in detail primarily in connection with Figs. 8 and 8A.
  • Because of the nature of centrifugal separation, . the first plasma that enters PRP bag 6 from whole blood bag 8 through tubing 52 is poor in platelets whereas the last plasma that enters PRP bag 6 is rich in platelets. These platelets (See Figs. 8 and 8A) tend to pool in bag 6 in the area labelled 804, close to the PRP input tube 52 which is adjacent the PPP output tube 54. Loss of these platelets from the PRP bag 6 could occur if they were allowed to mix with the rapid flow of PPP out of bag 6 through tube 54. This would result in a lower yield of platelets in the PRP bag 6 and a platelet contamination in the PPP bag 4.
  • Consequently, a barrier 802 is provided intermediate the PPP output port and the PRP input port. This barrier may be conveniently made by conventional heat or R.F. sealing during the fabrication of the bag 6. The barrier should preferably extend along the length of the bag from the input ports to about one inch from the bottom as shown by the vertically extending solid and dotted lines in Fig. 8.
  • With the barrier provided in PRP bag 8, the PPP must now circulate around the barrier. There'is, therefore, less disruption of the platelet concentrate in area 804 and platelets which are disrupted have a longer time to re-separate out as the plasma flows around the barrier 802.
  • Fig. 8 also shows a preferred embodiment of the apparatus for fixing the final volume of the platelet concentrate (PRP) left in PRP bag 6. A thin but rigid pressure plate 11, such as 0.060" thick aluminum, is disposed adjacent PRP bag 6 on the side nearest the center of rotation.
  • Pressure plate 11 is free to move radially against PRP bag 6 under the influence of centrifugal force. The plate 11 is of sufficient size to eclipse one side of bag 6. The other side of PRP Bag 6 abuts fixed support member 24. A flexible elastomeric gasket 806 is affixed to support member 24 of cassette 17 in a radial plane.
  • In operation, the PRP/PPP separation apparatus functions as follows:
    • After the PRP is separated and expressed/ siphoned to the PRP bag 6 and flow is automatically stopped from the whole blood bag _8 by the automatic pheresis valve mechanism 117, the centrifuge 2 continues to spin while the PPP tubing 54 is held clamped by the hydraulic timer mechanism 15 for a period of time sufficient to allow separation of platelets and PPP. The time and speed to produce separations depends on the diameter of the centrifuge rotor and location of the bags. In the embodiment shown, a rotor diameter of 11 inches and a speed of 2000 r.p.m. produced adequate separation of PRP into platelets and PPP within 2 minutes. Meanwhile, during the separation spin, the PPP tubing 54 is automatically filled with PPP priming the siphon between PRP bag 6 and PPP bag 4.
  • After the separation spin, PPP tubing 54 is unclamped. As separated PPP flows from the PRP bag 6, the bag tends to collapse and pressure plate 11 approaches the elastomeric gasket 806 and eventually compresses the PRP bag against the gasket forming a transverse barrier along the length of gasket 806 thereby preventing further flow out the PPP tube thus isolating the remaining plasma, which, for the reasons previously given, will be rich in platelets.
  • The location of the elastomeric gasket in relation to the height of the PRP bag 6 and the thickness of the gasket is adapted to isolate a predetermined volume of plasma in the PRP bag 6. For example, in the embodi- . ment of Fig. 8, 50 milliliters can be retained with a 1/16" ID by 1/8" OD tube gasket located one-third down the height of a 6" x 10" bag.
  • It should be noted that pressure plate 11 also functions to prevent formation of dynamic waves on the inner surface of the PRP bag 6. In addition, the mass of the pressure plate may be varied by adding or subtracting mass and thereby controlling the flow of PRP from the whole blood bag. A more massive pressure plate on the PRP bag in relation to the mass of the pressure plate on the whole blood bag 8 will decrease the rate of PRP flow since it will increase the back pressure on PRP bag 6.
  • Pressure plate 11 may also be fashioned with a section 803 cut out on the side opposite the PPP and PRP tubes 52 and 54. This cut out section 803 allows the PRP bag to bulge out within the cut out section. Since this bulge is pushed radially inward, any air 809 in PRP bag 6 will be pushed into the bulge and be isolated from the PPP output tube 54. This acts as a safety factor to prevent the vapor lock effect from occurring in tube 54.
  • After the PPP has been collected in PPP bag 4, clamps 31 and '35 of timer mechanism 15 clamp PRP tube 52 and PPP tube 54 and the centrifuge rotor is brought to rest. The end result of this process is a bag of packed RBC, a bag of PRP in bag 6 and a bag of PPP in bag 4.
  • This completes the overall system description of a first embodiment of the invention. What follows now is a description of further embodiments of the apparatus used in the invention.
  • Referring now to Figs. 9 and 10 (in which the numbers used are the same for parts corresponding to parts previously described in connection with Fig. 6) the effect of the size of the stopper ball 112 on the precise blood cut achieved is illustrated. In Fig..9, the ball stopper 112 has a relatively large diameter and tends to contact and seal outlet port 128 prior to the expulsion of all the first blood component l14. If the first blood component 114 is plasma and the second blood component 116 is packed red cells, the effect of the larger diameter ball stopper 112 is to lower the hematocrit of the second blood component remaining in the blood processing bag 8. On the other hand, when a relatively smaller diameter ball stopper is employed, such as in Fig. 10, a much smaller amount of PRP 114 remains in the flexible blood processing bag 8. Thus, the hematocrit of the second blood component or packed red cells 116 is raised.
  • Fig. 11 shows a further embodiment of a Pheresis Valve for sealing the outlet port of a flexible blood processing bags. In this embodiment, a hinged flap 110 has one end joined to an interior surface of the flexible blood-processing bag 8 at a position adjacent to the outlet port 128. The hinged flap 110 is of a density similar to that of the stopper ball 112 and operates in a manner.similar to the stopper ball 112 previously described in that it floats at the interface between first blood component 114 and second blood component 116. Thus, as this interface approaches the outlet port, the hinged flap is carried' into contact with the outlet port 128 thereby creating the required seal.
  • In some applications of the invention, such as cell washing or gaining maximum plasma yield, it is desirable to be able to re-open the Pheresis Valve 117 after it closes. In the embodiments heretofore described, once the valve closes, it is prevented from re-opening by the high negative pressure of the fluid downstream (in the direction C of Fig, 6) from the valve.
  • One way to make the valve re-open is to minimize the negative pressure force in the direction C of Fig. 6 and maximize the positive buoyancy force in the opposite direction created by the volume of fluid left in the bag 8. This could be accomplished by decreasing the cross-sectional area of the output tube 52 and increasing the size and therefore the buoyant volume of the valve float. The latter is undesirable since it increases the manufacturing cost of the bag and the former increases the disruptive shear stresses of blood components flowing through the valve, thereby increasing the probability of occlusions.
  • A better solution to this problem is shown in Fig. 12 which is a cross-sectional view taken along the lines 12-12 of Fig. 7. As shown in Fig. 12, the valve seat 122 is made leaky by one or more tiny slots 212 on the valve seat 122 so that the negative downstream pressure is dissipated. The slots leak about 1 millilitre per minute when the ball valve is seated.
  • The operation of the slotted valve may be described as follows, in connection with Figs 9 and 12:
    • First, the ball stopper 112 approaches the valve seat 122 as it floats on the interface between RBC 116 and plasma 114. Eventually, the ball stopper 112 lodges in the valve seat and cuts off the flow of plasma 114 through PRP tubing 52. As the centrifuge continues to spin, more plasma 114 is separated from whole blood and the interface between plasma and RBC moves away from the valve seat. At the same time, some of the plasma 114 leaks through the slits 212 into the output tube 52 dissipating the negative pressure on that side of the ball stopper. At some point, the buoyancy force on the stopper 112 becomes greater than the negative pressure in the tube 52 and the valve mechanism 117 re-opens allowing the flow of plasma to resume. The apparatus may be permitted to re-cycle as described above until substantially all the plasma is separated from the whole blood.
  • A further embodiment of the invention in which the PRP bag pressure plate 1-1 is eliminated is shown in Figs. 13 and 14. In the embodiment shown in Figs. 13 and 14, the PRP input port for tubing 52 and output port for PPP tubing 54 are located at the top of PRP bag 6. The timer clamp 15 is located as close to rotor housing 34 as possible. The inner diameter of the PPP tubing 54 is large enough so that the capillary air bubble surface tension inside the tube is less than the centrifugal force'pressure on the fluid in the tube.
  • Initially, the PPP tube 54 and bag 4 are empty. As plasma is expressed into the PRP bag 6, the air in the PPP tubing 54 is locked by the plasma. However, the air surface in the tube 54 cannot withstand the outward pressure of the plasma and this air is displaced out of the PPP tubing 54 into bag 6.
  • After the platelets are settled out of the plasma in PRP bag 6 and become deposited on the outer wall of bag 6, the tubing 54 is unclamped by clamp 35 of timer 5 and PPP is siphoned from PRP bag 6 into PPP bag 4. Ramp 300 is provided on partition wall 24 adjacent the exit port for PPP tubing 54 on bag 6. The separated platelet concentrate in bag 6 is substantially prevented from exiting the PRP bag 6 by this ramp. A mass clamp 302, such as a 1.27 mm thick strip of plastics, may be disposed adjacent the inner wall of bag 6 opposite the ramp and near the outlet to PPP tubing 54. This mass clamp 302 will terminate PPP flow at a predetermined volume. Such volume may, for example, be at a ratio of 50 ml of plasma for each single unit platelet concentrate left in PRP bag 6 as presently specified by clinical standards.
  • By proper design of the angle of inclination of ramp 300 and its location and the weight and location of mass 302, flow may be terminated at this 50 ml level. The clamp mass 302 has very little influence on the PRP bag 6 until sufficient PPP has been siphoned out of the bag thereby bringing the inner walls of the bag close together, i.e., within 0.254mm.
  • When this occurs, negative Bernoulli pressure due to the high flow rate of PPP out tubing 54 pulls the two inner walls of bag 6 together, terminating flow. Once the flow ceases, the negative pressure (previously described) from the siphon effect is large enough to keep the walls of the bag 6 under the clamp mass sealed together.
  • Instead of locating the first blood processing bag nearer to the center of rotation than the second bag (which as aforesaid may merely be a rigid receptacle for receiving separated components) as in the embodiments heretofore illustrated, it may be desirable to have a "side-hv-side" arrangement in which the first and second bags are located along the periphery or the rotor housing equidistant to the center of rotation as giagrammatically illustrated in Fig. 15
  • In the embodiment of Fig. 15, a centrifuge 140 of the type previously described, rotates about a center of rotation labelled "CR". The centrifuge rotor housing 142 supports two flexible bags 144 and 146 in a vertical position on the periphery of the rotor and equidistant from the center of rotation.
  • A contoured framework 150 with concave inwardly extending surfaces, allows bag 144 to rest naturally against the housing inner surface with a minimum of stress on the bag wall material when subjected to centrifugation. Alignment pins (not shown) keep the bag 144 properly oriented. Inner wall 152 of bag 144 is essen- .tially free-standing except for a light weight, stiff, curved pressure plate 148 disposed against the surface of inner wall 152 so as to produce a liquid pressure in the bag when subjected to the centrifugal field.
  • Interconnecting tubing 154 is provided between the exit port of first bag 144 and the second bag 146 (in this case the receiver container). This tubing passes over a curvilinear contour (or dam) 156 which may be incorporated into the framework 150.
  • This contour is sufficiently large to assure that the exit port of bag 144 is at a lesser distance from the center of rotation than any other portion of the bag 144. Furthermore, the shape of the container is such that the fluid pathway in the first bag near the exit port is in the form of an approach ramp with gradually decreasing radius for locations progressively closer to the exit port.
  • The second bag 146 is merely a receiving container for the separated component from the first bag. The volume of this container is pre-established to just accomodate the volume of separated component (supernatant) desired to be recovered from bag 144. Suitable support means (not shown) hold bag 146 in place against rotor housing 142. Flow from bag 144 to bag 146 is terminated by setting the volume of the second bag 146 so that it is filled completely before all the supernatant has passed from the first bag 144.
  • For high yield application, for example, in the separation of plasma from whole blood, an accurate predetermination would be required of the volume of supernatant to be expected from the separation as, for example, by determining the hematocrit of the anticoagulated whole blood when preparing for separation of whole blood into plasma and RBC. Another
  • way of providing an accurate automatic cut is to select a pressure plate 148 with a weight sufficient to force supernatant, such as plasma, over into the receiver container (bag 146) but not great enough to force the more dense components such as RBC into bag 146.
  • The pressure in the first bag is proportional to the difference between the squares of the radii to the input and output of the fluid column, to the density of the fluid in the column, and to the square of the rotatinq speed.
  • The density of packed RBC is about 1.10, whereas the density of the supernatant plasma is about 1.03. Greater pressure is therefore required to force red cells radially inward to a given radial point than is required to force plasma at this point. Therefore, when the cut is being made, flow from bag 144 to bag 146 will automatically cease when RBC pass part of the way through the radial passage 154 to the second bag 146, provided the weight of prcs- sure plate 148 is suitably matched to the process.
  • As in the earlier described embodiments, it is important that, to make a clean separation, it is necessary to run the centrifuge long enough to generate clear supernatant before allowing any flow to occur through the interconnecting pathway 154 between the first bag 144 and second compartments 146. In other words, it is necessary to avoid a situation in which the fluid in the interconnecting pathway 154 is close to the density of supernatant but still has some cells suspended in it. Thus, it is evident that the operating protocol must include a first period of centrifugation while the interconnecting tubing is clamped shut as by the previously described timer mechanism 15 or equivalent. Then the clamp may be opened and clear supernatant may be passed over into the bag in the second compartment 146 until packed RBC flow part way through the interconnecting pathway.
  • Fig. 16 is an improved version of the Fig. 15 apparatus wherein the pressure plate 148 is made large enough in surface area to cover the entire area of wall surface 152 of first blood processing bag 144, thus no bulging is possible. Additionally, the center of gravity of pressure plate 148 is off-centered slightly to a point labelled 164; thereby automatically providing a more optimal separation zone. The center of gravity may be off-set by contouring the shape of plate 148 or by adding or subtracting material from the plate as required. The dam or ramp 156 previously located on the rotor housing is now located on the pressure plate 152 and moves with the plate thereby providing a more constant ramp function.
  • In summary, in the apparatus described in connection with Fig. 16, no specialized contoured outer shoe and frame is necessary. Instead, the blood processing bag 144 can be simply inserted against the inner wall 142 of the rotor. An optimal separation compartment is automatically created by use of a pressure plate 148 with an off-centered center of gravity. Alterations in the separation zone can be made very simply by merely adding or repositioning tiny weights (not shown) on the pressure plate 148.
  • It should be understood that while only two bags are used for illustration in Figs. 15-16, the separation process may be extended in a variety of ways as shown for example in Fig. 17 by adding a pressure plate 180 on bag 146 and interconnecting bag 146 over a second dam 184 to a third bag 182. A process similar to the three bag pheresis process described in connection with Figs. 1-8 may then be carried out by clamping the interconnecting tubing with clamps 185 and 187 at appropriate intervals and centrifugally separating RBC and plasma from whole blood in bag 144. The plasma is then expressed to bag 146 by means of a pressure plate 148 having a mass just sufficient to express the lighter weight plasma sideways over the dam 156 and into bag 146. Next, the plasma in bag 146 is centrifugally separated into PRP and PPP. Finally, the PPP is expressed sideways over the second dam 184 by the force of pressure plate 180 which is preestablished so as to express all but a fixed volume of fluid, for example 50 ml, into the fhird bag 182.
  • The clamps 185 and 187 may be controlled by a hydraulic timer mechanism as described earlier.
  • A typical procedure is as follows:
    • 1) Whole blood is contained in bag 144, clamps 185 and 187 are closed to prevent flow. The centrifuge 140 spins at a low r.p.m. of about 1000 r.p.m. for a few minutes.
    • 2) Clamp 185 opens and allows plasma to flow into bag 146.
    • 3) Clamp 185 closes and the rotor speed increases to two or three times the low r.p.m. for a few minutes.
    • 4) Clamp 187 opens and cell-free plasma PPP flows into bag 182.
    • 5) Clamp 187 closes and the centrifuge stops.
  • Another application of the invention' is shown in the embodiment of Fig. 18 which illustrates red blood cell washing apparatus. In Fig. 18 three flexible bags 190, 192, and 194 are disposed about the periphery of the rotor housing 142 of centrifuge 140 equidistant from the center of rotation CR. Bag 190 contains a washing solution, such as a solution of sterile saline. Bag 194 is interconnected with bag 190 by tubing 196 and with spent solution bag 192 by tubing 198 which extends over dam 195. Clamp means 191 and 193 operated by a timer mechanism (not shown) control the flow of fluid through respective tubing 196 and 198. :
  • Bag 194 is substantially similar to the blood processing bags previously described. It contains the whole blood or thawed glyceralized blood to be washed.
  • A typical procedure is as follows:
    • 1) Clamps 191 and 193 are closed and the centrifuge 140 is brought up to a running speed of about 2000 r.p.m. for a few minutes.
    • 2) Clamp 193 is opened and separated plasma and/ or freezing solutions and saline are expressed from bag 194 through tubing 198 into the spent wash solution bag 192 by the pressure generated by the pressure plate 197.
    • 3) Clamp 193 is closed and clamp 191 is opened, filling the.blood processing bag with wash solution. Clamp 193 then closes.
    • 4) The centrifuge is then spun for a pre-ceter- mined time period or stopped and agitated to mix the blood/wash solution mixture for a time period (similar to the conventional washing machine agitation cycle) and then brought up to a.speed of 2000 r.p.m. for a period of time.
    • 5) Clamp 193 is then opened and the pressure plate 197 expresses the spent wash solution from bag 194 into bag 192, as the rotor spins.
    • 6) This procedure would be repeated a number of times until adequate washing has taken place.
  • The final product of this procedure is a unit of packed washed red cells. The hematocrit of the packed cells can be made very high. The clamps for this procedure may-be controlled by the hydraulic timer clamp mechanism previously mentioned.
  • An alternative to the procedures heretofore described for controlling the flow of fluids between first and second bags is shown in the embodiment of Fig. 19. In this embodiment opto/electronic/ mechanical means are employed in place of, for example, the hydraulic timer and pheresis valve components previously mentioned.
  • The apparatus described in Fig. 19 is illustrated in connection with the present apparatus, however, the invention described in this embodiment may be applied to a variety of blood processing apparatus and methods.
  • In the simplified schematic of Fig. 19, the interconnecting tubing 52 between whole blood bag 8 and PRP bag 6 is shown disposed between a light transmitter element 250 and photo-detector 252 of a well-known beam optical sensor 260. Beam sensor 260 may alternatively comprise a simple reflective optical beam sensor. Tubing 52 also passes between a solenoid activated flow clamp 254.
  • When fluid in tubing 52 changes color, such as when all the plasma (yellow in color) has passed through the tubing 52 from whole blood bag 8 as a result of the centrifugally induced siphon effect previously described, a change in voltage will occur at the output lead of photodetector 252 as the red colored RBC's start to pass. The color change is sensed by the photodetector 252 which generates a voltage signal. This voltage signal is coupled to power supply/ control module 258 which-in turn energizes the coils of a solenoid mounted on clamp 254 thereby causing the clamp to stop the flow through tubing 52.
  • Thus, when the flow from the blood processing bag 8 turns from yellow to red, the component line 52 will be clamped. This will trap the RBC's in the whole blood bag 8 and the plasma in the PRP bag 6. Similar apparatus can be used to sense the color change between PPP and PRP to actuate an additional clamp on the tubing 54 between the PRP bag and PPP bag.

Claims (35)

1. Apparatus for use in the centrifugal separation of blood into at least a first blood component and a second blood component comprising:
a flexible blood processing bag (8;144) for containing anticoagulated whole blood and having an outlet port;
a receiving container (6;146) for receiving a component of said whole blood and having an input port; and tubing means providing fluid communication between the output port of the bag and the input port of the receiver container; characterised by valve means (117; 154, 156; 156,185) for terminating flow of fluid component out the output port of the bag (8; 144) in response to the specific gravity of said component.
2. The apparatus of claim 1, in which the valve means prevents fluid communication between said flexible blood processing bag and said receiver container in response to the difference between the specific gravities of separated first and second blood components.
3. The apparatus of claim 2, in which said valve means comprises a stopper (112) having a specific gravity which is lower than the specific gravity of first blood component (114) but higher than the specific gravity of second blood component (116).
4. The apparatus of claim 3, in which said stopper is contained within a guide (119) located at the outlet port (128) of said flexible blood processing bag.
5. The apparatus of claim 4, in which said , guide includes means (212) for preventing sealing of said outlet port caused by the flow of first blood component through said port.
6. The apparatus of claim 5, in which said means for preventing sealing comprise flow passages in said guide located between said outlet port and the normal resting position of said stopper.
7. The apparatus of claim 3, in which said stopper comprises a flap (110) connected to the interior surface of said flexible blood processing bag adjacent to said outlet port (128).
8. Apparatus for processing fluids in a centrifugal force field to separate constituent components of such fluids comprising in combination:
a centrifuge (2;140) having a rotor adapted to rotate at a sufficient speed to cause said components to separate; a flexible bag (8;144;194) for containing
a first fluid; and a receiver container (6;146;192) for receiving at least one component of said first fluid; characterised by mass means (10;148;180;197) disposed nearer the center of rotation of the rotor than the flexible bag and adapted to move and contact
a surface of said bag, said mass being sufficient to at least initiate a flow from said bag to said container of component fluid separated in said bag.
9. The apparatus of claim 8, in which the bag (144;194) and container (146;192) are located on the rotor substantially equidistant from the center of rotation.
10. The apparatus of claim 8, in which the force exerted by the mass means is just sufficient to force the component with the least specific gravity from the bag to the container.
11. The apparatus of claim 8, in which the bag (8) is located radially inward from the container (6).
12. The apparatus of claim 8, in which control means (117;156,154;156,185;184,187)-are provided for stopping the flow of fluid when substantially the entire volume of fluid component of a predetermined characteristic has left said bag.
13. The apparatus of claim 12, in which the characteristic of the fluid is an optical property.
14. The apparatus of claim 13, in which the control means is electrically actuated.
15. The apparatus of claim 12, in which the characteristic of the fluid is specific gravity.
16. The apparatus of claim 8, in which clamp means (15;185:1877193) are provided to prevent fluid flow from said bag to said container until a predetermined level of fluid processing has been achieved by rotation of said rotor.
17. The apparatus of claim 8, in which red blood cells are washed in the flexible bag and the component fluid which flows to the container is spent wash solution.
18. The apparatus of claim 8, in which whole blood is separated in the flexible bag and the component fluid which flows to the container is plasma.
19. The apparatus of claim 18, including control means (117;156,154;156,185) for stopping the flow to the container when substantially all the plasma has left the bag.
20. The apparatus of claim 19, in which the control means comprises a valve (117) controlled by the specific gravity of fluid flowing from the flexible bag.
21. The apparatus of claim 20, in which the valve means comprises a float valve.
22. The apparatus 8, in which platelet rich plasma is separated in the flexible bag and the component fluid which flows to the container is platelet poor plasma.
23. The apparatus of claim 8, in which the receiver container.is a flexible bag (6;146) with an inout port and an output port and a second receiver container (4) is coupled to the output port to receive a fluid component separated in the first said receiver container.
24. The apparatus of claim 23, in which PRP and RBC are separated in the first flexible bag and the PRP flows to the first said receiver container where the platelets are separated and PPP flows to the second receiver container while the platelets remain.
25. The apparatus of claim 23 or 24, in which valve means (117;154,156) are provided to prevent flow after fluid component separation is achieved in said first said container.
26. The apparatus of claim 25, in which the valve means comprises a float valve (110;112) having a float with a specific gravity intermediate that of the components being separated.
27\ The apparatus of claim 8, in which the receiver container (6;146) is also flexible and a second mass means (11;180) is movably disposed adjacent thereto nearer the center of rotation of the rotor than said receiver container.
28. A method'in which blood is centrifugally separated into a first blood component (114) and second blood component (116) in a blood processing chamber (8;144) and first blood component is thereafter caused to flow through an outlet port (128) of said chamber through a conduit and into a receiver container (6;146) characterised by causing said flow by a weight (10;148) disposed adjacent said chamber.
29. The method of claim 28, in which flow is stopped to the container with a valve means (117) having a stopper (110;112) with a specific gravity which allows it to float on the interface between first and second blood components within said chamber.
30. The method of claim 28, in which the conduit (52B) between said chamber and container has an inner diameter (ID2) sufficiently small to cause the second blood component to achieve a flow velocity which will cause any air bubbles in the conduit to flow to said container.
31. The method of claim 28, in which the first blood component is plasma and the second component is red blood cells.
32. The method of claim 28, including rotating a volume of whole blood contained in a first flexible bag (8;144) in a centrifuge at a speed sufficient to separate said whole blood into at least a less dense and more dense componentand forcing the less dense component to flow from said bag to a container (6;146) by applying centrifugal force to a movable body (10;148) of fixed weight in direct contact against a planar surface of said bag while said volume is being rotated, the flow of less dense component from said bag to said container being prevented until substantial separation of the whole blood in said first flexible bag has occurred and said flow being caused to stop when the less dense component has passed from the bag to the container.
33. The method of claim 32, in which the flow is caused to stop by control means (117;156,54) responsive to the density of one of said components.
34. The method of claim 32, in which the flow is caused to stop by providing the movable body (148) with enough weight to displace the less dense component and not the more dense component.
35. The method of claim 32, in which the flow is caused to stop by a sensor (252,260) responsive to optical change as different blood components pass the sensor.
EP19820303594 1981-07-09 1982-07-08 Centrifuging apparatus and methods for separating fluids into components thereof Expired EP0070159B1 (en)

Priority Applications (1)

Application Number Priority Date Filing Date Title
AT82303594T ATE31033T1 (en) 1981-07-09 1982-07-08 CENTRIFUGE APPARATUS AND PROCESS FOR THE DIVISION OF LIQUIDS INTO THEIR COMPONENTS.

Applications Claiming Priority (4)

Application Number Priority Date Filing Date Title
US281655 1981-07-09
US06/281,655 US4421503A (en) 1981-07-09 1981-07-09 Fluid processing centrifuge and apparatus thereof
US281649 1981-07-09
US06/281,649 US4402680A (en) 1981-07-09 1981-07-09 Apparatus and method for separating fluid into components thereof

Publications (3)

Publication Number Publication Date
EP0070159A2 true EP0070159A2 (en) 1983-01-19
EP0070159A3 EP0070159A3 (en) 1984-07-04
EP0070159B1 EP0070159B1 (en) 1987-11-25

Family

ID=26961012

Family Applications (1)

Application Number Title Priority Date Filing Date
EP19820303594 Expired EP0070159B1 (en) 1981-07-09 1982-07-08 Centrifuging apparatus and methods for separating fluids into components thereof

Country Status (5)

Country Link
EP (1) EP0070159B1 (en)
AU (1) AU8565682A (en)
DE (1) DE3277722D1 (en)
DK (1) DK306582A (en)
ES (1) ES513812A0 (en)

Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
EP0935998A1 (en) * 1998-02-17 1999-08-18 Andreas Hettich GmbH & Co. KG Centrifuge and blood bag with pressure chamber and blood chamber

Families Citing this family (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US4900298A (en) * 1987-08-21 1990-02-13 Cobe Laboratories, Inc. Centrifuge drive and support assembly
AU587949B2 (en) * 1987-08-26 1989-08-31 Cobe Laboratories Inc. Sterile blood component collection
EP2883616A1 (en) * 2013-12-11 2015-06-17 Alfa Laval Corporate AB Valve for draining off gas from a centrifugal separator
CN109569900B (en) * 2019-01-25 2023-12-22 中国工程物理研究院总体工程研究所 Self-balancing device of geotechnical centrifuge

Citations (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US3648697A (en) * 1969-08-01 1972-03-14 Gardner Newell J Intravenous feeding container and method of preparing the same
FR2152741A1 (en) * 1971-09-07 1973-04-27 Corning Glass Works
US4010894A (en) * 1975-11-21 1977-03-08 International Business Machines Corporation Centrifuge fluid container
EP0014093A1 (en) * 1979-01-22 1980-08-06 Haemonetics Corporation An apparatus, a method and a disposable blood pathway for use in separating blood into components thereof
EP0026417A2 (en) * 1979-09-22 1981-04-08 Firma Andreas Hettich Centrifuge with system of bloodbag for the separation of blood components

Patent Citations (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US3648697A (en) * 1969-08-01 1972-03-14 Gardner Newell J Intravenous feeding container and method of preparing the same
FR2152741A1 (en) * 1971-09-07 1973-04-27 Corning Glass Works
US4010894A (en) * 1975-11-21 1977-03-08 International Business Machines Corporation Centrifuge fluid container
EP0014093A1 (en) * 1979-01-22 1980-08-06 Haemonetics Corporation An apparatus, a method and a disposable blood pathway for use in separating blood into components thereof
EP0026417A2 (en) * 1979-09-22 1981-04-08 Firma Andreas Hettich Centrifuge with system of bloodbag for the separation of blood components

Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
EP0935998A1 (en) * 1998-02-17 1999-08-18 Andreas Hettich GmbH & Co. KG Centrifuge and blood bag with pressure chamber and blood chamber

Also Published As

Publication number Publication date
ES8401322A1 (en) 1983-12-01
EP0070159A3 (en) 1984-07-04
AU8565682A (en) 1983-01-13
ES513812A0 (en) 1983-12-01
EP0070159B1 (en) 1987-11-25
DE3277722D1 (en) 1988-01-07
DK306582A (en) 1983-02-08

Similar Documents

Publication Publication Date Title
US4421503A (en) Fluid processing centrifuge and apparatus thereof
US4402680A (en) Apparatus and method for separating fluid into components thereof
EP0014093B1 (en) An apparatus, a method and a disposable blood pathway for use in separating blood into components thereof
US4482342A (en) Blood processing system for cell washing
EP1161269B1 (en) System for collecting platelets and other blood components
US4285464A (en) Apparatus for separation of blood into components thereof
US5779660A (en) Blood collection and separation process
AU581458B2 (en) Closed hemapheresis system and method
US6261217B1 (en) Separation set having plate-like separation container with annular pinch valve for blood component preparation
US4269718A (en) Process and device for centrifugal separation of platelets
US4445883A (en) Deformable support for fluid processing centrifuge
EP0765687A1 (en) Method for centrifugal blood processing
EP2815776B1 (en) System for blood separation with gravity valve for controlling a side-tapped separation chamber
US20060116271A1 (en) Continuous blood separator
EP0070159B1 (en) Centrifuging apparatus and methods for separating fluids into components thereof
AU718172B2 (en) Method of collecting and processing blood
GB2075376A (en) Process and device for centrifugal separation of platelets

Legal Events

Date Code Title Description
PUAI Public reference made under article 153(3) epc to a published international application that has entered the european phase

Free format text: ORIGINAL CODE: 0009012

AK Designated contracting states

Designated state(s): AT CH DE FR GB IT LI NL SE

PUAL Search report despatched

Free format text: ORIGINAL CODE: 0009013

AK Designated contracting states

Designated state(s): AT CH DE FR GB IT LI NL SE

17P Request for examination filed

Effective date: 19841212

17Q First examination report despatched

Effective date: 19860319

GRAA (expected) grant

Free format text: ORIGINAL CODE: 0009210

RAP1 Party data changed (applicant data changed or rights of an application transferred)

Owner name: LATHAM LABS. INC.

RAP1 Party data changed (applicant data changed or rights of an application transferred)

Owner name: HAEMONETICS CORPORATION(A MASSACHUSETTS CORPORATIO

AK Designated contracting states

Kind code of ref document: B1

Designated state(s): AT CH DE FR GB IT LI NL SE

PG25 Lapsed in a contracting state [announced via postgrant information from national office to epo]

Ref country code: NL

Effective date: 19871125

Ref country code: LI

Effective date: 19871125

Ref country code: IT

Free format text: LAPSE BECAUSE OF FAILURE TO SUBMIT A TRANSLATION OF THE DESCRIPTION OR TO PAY THE FEE WITHIN THE PRESCRIBED TIME-LIMIT;WARNING: LAPSES OF ITALIAN PATENTS WITH EFFECTIVE DATE BEFORE 2007 MAY HAVE OCCURRED AT ANY TIME BEFORE 2007. THE CORRECT EFFECTIVE DATE MAY BE DIFFERENT FROM THE ONE RECORDED.

Effective date: 19871125

Ref country code: CH

Effective date: 19871125

Ref country code: AT

Effective date: 19871125

REF Corresponds to:

Ref document number: 31033

Country of ref document: AT

Date of ref document: 19871215

Kind code of ref document: T

PG25 Lapsed in a contracting state [announced via postgrant information from national office to epo]

Ref country code: SE

Effective date: 19871130

REF Corresponds to:

Ref document number: 3277722

Country of ref document: DE

Date of ref document: 19880107

ET Fr: translation filed
REG Reference to a national code

Ref country code: CH

Ref legal event code: PL

NLV1 Nl: lapsed or annulled due to failure to fulfill the requirements of art. 29p and 29m of the patents act
PLBE No opposition filed within time limit

Free format text: ORIGINAL CODE: 0009261

STAA Information on the status of an ep patent application or granted ep patent

Free format text: STATUS: NO OPPOSITION FILED WITHIN TIME LIMIT

26N No opposition filed
PG25 Lapsed in a contracting state [announced via postgrant information from national office to epo]

Ref country code: GB

Effective date: 19890708

GBPC Gb: european patent ceased through non-payment of renewal fee
PG25 Lapsed in a contracting state [announced via postgrant information from national office to epo]

Ref country code: FR

Free format text: LAPSE BECAUSE OF NON-PAYMENT OF DUE FEES

Effective date: 19900330

PGFP Annual fee paid to national office [announced via postgrant information from national office to epo]

Ref country code: DE

Payment date: 19900330

Year of fee payment: 8

REG Reference to a national code

Ref country code: FR

Ref legal event code: ST

PG25 Lapsed in a contracting state [announced via postgrant information from national office to epo]

Ref country code: DE

Effective date: 19910403