CN1536077A - High-yield recombinant influenza B virus strain and its application - Google Patents
High-yield recombinant influenza B virus strain and its application Download PDFInfo
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Abstract
The present invention relates to a kind of new influenza B virus complete gene sequence with mammalian cell high-yield characteristics and carrier containing said equence and strain. Said invention also relates to the influenza B vaccine prepared by using the described strain.
Description
Technical field
The present invention relates to reorganization Influenza B virus strain of a kind of high yield and uses thereof, and the nucleic acid of this virus stain of recombinating and primer, particularly the second type influenza virus vaccine for preparing via this strain.
Background technology
Influenza is a kind of respiratory tract disease that is caused by influenza virus.According to " science " magazine, in influenza season occurred frequently, because the labor force reduces and the medical expense increase, the financial loss of bringing to the U.S. is above 12,000,000,000 dollars.In addition, annual all have the American more than 20,000 to die because of influenza.
The influenza storm that have swept the globe in 1918 causes 2,000 ten thousand-4,000 ten thousand people's death altogether, surpasses the summation of death toll in the World War I.The influenza that the last time is swept away the whole world occurs in nineteen sixty-eight, has seized nearly 500,000 people's in the whole world life, and wherein the overwhelming majority is the elderly, and still, also having many once was the healthy young people.Flu outbreak is because fatal virus variant occurred.And Britain's " nature " magazine claims, such deadly virus variation occurred once in average per 30 years to 40 years.This danger was shown indications of a new development in 1997.That year, there are 18 people in Hong Kong by a kind of avian influenza, and 6 people die.In May calendar year 2001, avian influenza virus has been found in Hong Kong again, although virus this time is considered to can not infect the mankind, the Hongkong government still do not stint the loss 2.45 hundred million Hongkong dollars, put to death about 1,300 ten thousand poultry.
Avoid influenza to break out again, the most important thing is, in time discover viral fatal variation and prepare corresponding vaccine.WHO has started global influenza monitoring network from 1948.In every year, WHO will gather the popularity of various countries' influenza virus strain, analyzes next year possibility popular Virus Type then, and announces conclusion in 6 months in advance, and each producer then produces vaccine on this basis.Although many people think that this network is effective, working efficiency that it is present and research level can not guarantee to make when in a single day viral fatal mutation occurs accurately and rapidly reaction.
Influenza virus worldwide causes people and animals' morbidity and death.The popular Chang Youjia and the Influenza B virus of influenza cause, the surface antigen of influenza virus is important component part (the Jackson D of influenza vaccines, CadmanA, Zurcher T, Barclay WS.A reverse genetics approach for recovery ofrecombinant influenza B viruses entirely from cDNA.J Virol.2002Nov; 76 (22): 11744-7).But, influenza virus is because antigen conversion or antigenic drift often cause the appearance of new variant antigens, therefore vaccine strain need often be replaced (Hoffmann E, Mahmood K, Yang CF, Webster RG, Greenberg HB, Kemble G.Rescue of influenza B virus from eightplasmids.Proc Natl Acad Sci U S is Aug 20 A.2002; 99 (17): 11411-6).Currently get the Green Light that what produce is the inactivated vaccine in chicken embryo source,, still exist many deficiencies although take effective viral purification technology.Not only need a large amount of chicken embryos, and the production cycle is long.The vaccine that produces in tissue culture has been obtained reasonable protectiveness (Govorkova EA in animal model, Murti G, Meignier B, de Taisne C, Webster RG.African green monkey kidney (Vero) cells provide an alternative host cell system for influenza A and B viruses.J Virol.1996 Aug; 70 (8): 5519-24).At present, the mammalian cell mdck cell is considered to cultivate first type and the only clone of Influenza B virus (Robertson JS.Related Articles, Links An overview of host cell selection.Dev Biol Stand.1999; 98:7-11; Discussion 73-4), this clone has the back of infection and produces influenza virus rapidly, obtains the characteristics of high titre at short notice.The virus in MDCK source is through after the continuous passage in addition, kept antigenic stability (Govorkova EA, Kodihalli S, Alymova IV, Fanget B, Webster RG.RelatedArticles, Links Growth and immunogenicity of influenza viruses cultivatedin Vero or MDCK cells and in embryonated chicken eggs.Dev Biol Stand.1999; 98:39-51; Discussion 73-4).
Yet not every virus all is adapted in some cell growth and can becomes vaccine strain, and for example some viruses output in chicken embryo and/or mammalian cell is very low.Therefore, the problem that solves is the reassortant that obtains high yield, the method that adopts is that the HA and the NA fragment of breadboard high yield strain that has obtained and epidemic isolates are carried out reprovision at present, make vaccine strain both keep the characteristic of high yield, has the antigenic characteristics of epidemic isolates (Hoffmann E again, Mahmood K, Yang CF, Webster RG, Greenberg HB, Kemble G.Rescueof influenza B virus from eight plasmids.Proc Natl Acad Sci U S A.2002Aug 20; 99 (17): 11411-6).
The development of reverse genetic technology makes quick acquisition influenza vaccines become possibility.On the basis of the female strain of high yield of recombinating out, obtain vaccine strain and only need simple clone, and rotaring dyeing technology, the time that approximately needed for two weeks, need 2 months time and obtain recombinant virus, therefore obtain the production time that vaccine strain has greatly shortened vaccine with the reverse genetic method with classical reallocating method.Neuman (Gabriele Neumann and Yoshihiro Kawaoka, 1Virology 287,243 ± 250 (2001)) is defined as the process that is produced strand RNA by cDNA with the antisense genetic technique, be participated in by the RNP mixture.A plurality of stages have been experienced in the development of this technology.1989, help viral system to produce.Palse research group has set up the system of first research minus-stranded rna virus, has started from the clone
cDNA produces reorganization
vIn new era of RNA, created the RNP transfection method.Hobom and Colleagues (Neumann, G., Zobel, A., and Hobom, G. (1994) .RNA polymerase I-mediated expression of influenza viral RNAmolecules.Virology 202,477 ± 479.) push away and go a step further, first Application RNA Polymerse1 and Helper virus system.
The characteristics of Polymerse1 show as:
1, Polymerse1 transcribes rRNA and does not comprise 5 ' cap and 3 ' stern construction, utilizes this point can transcribe out viral genome.
2, can not prolong transcriptional domain with the promotor and the terminator of length-specific, guarantee that the advantage of virus genomic integrity Polymerse1 system is more convenient than RNP transfection method, do not need in-vitro transcription, the assembling of protein purification and RNP.
But it should be noted that above two systems all exist shortcoming: promptly yield poorly, generation be defective virus mostly.Help viral background height, need a large amount of screening operations.Make the practicality of this technology seem not enough.So in 1994, people such as Conzelmann (Schnell, M.J., Mebatsion, T., and Conzelmann, K.K. (1994) .Infectious rabies viruses from cloned cDNA.EMBO J.13,4195 ± 4203.) with the t7 rna polymerase systems produce rabies virus.Neuman (Neumann, G., Watanabe in 1999, T., Ito, H., Watanabe, S., Goto, H., Gao, P., Hughes, M., Perez, D., Donis, R., Hoffmann, E., Hobom, G., and Kawaoka, Y. (1999) .Generationof influenza A viruses entirely from cloned cDNAs.Proc.Natl.Acad.Sci.96,9345 ± 9350.) etc. the people has successfully cloned influenza virus, and they have adopted the method for 12 plasmid co-transfections, wherein 8 plasmids are transcribed out viral genome segment respectively, 4 albumen that plasmid expression is relevant with virus replication with these 12 plasmid co-transfection mammalian cells, have obtained recombinant virus particle.The shortcoming of this system is that 12 plasmid co-transfections have increased the difficulty of transfection, have limited the use of clone.After this Hoffmann (HoffmannE, Stech J, Guan Y, Webster RG, Perez DR.Universal primer set for thefull-length amplification of all influenza.A viruses.Arch Virol2001; 146:2275-89.) invented 8 pUC pUCs on this basis, can not only transcribe out the full gene group of virus, can also give expression to all viral proteins, utilize this system, successfully packed out influenza virus.
The genomic characteristics of Influenza B virus are the member of orthomyxoviridae family as influenza A virus, are made up of 8 segmented strand RNAs.Generally speaking, the Influenza B virus encoded protein is similar to the first type, its the 6th and the 7th fragment shows specific characteristics, described the 6th sections coding NA and NB albumen, proteic function of NB and M2 protein similar, perhaps, the 7th sections coding M1 and BM2 albumen, the difference of the characteristic in these heredity help to understand the host range restriction of Influenza B virus and the difference of other character.
Influenza B virus is divided into Yamagata system and Victoria system according to the difference in HA1 district, and their common feature is the conserved regions that 9 bases are arranged at virus genomic 3 ' and 5 ' end, and 10,11 be (the seeing Table) of relative variation.(conserved regions of 3 ' and 5 ' terminal 9 bases of influenza virus shows with thick surplus matrix, HA wherein, and NA, the 6th of the segmental 5 ' end of NS is that the 6th of all the other fragment of T are A).
This shows, seek the Influenza B virus maternal plant of a high yield, the clone who obtains its whole 8 gene fragments carries out reprovision with the HA and the NA fragment of high yield strain gene and epidemic isolates then, make vaccine strain both keep the characteristic of high yield, have the antigenic characteristics of epidemic isolates again, preparing the second type influenza virus vaccine like this, will be the major transformation that influenza vaccines produce.
Summary of the invention
In order to overcome the deficiencies in the prior art part, the object of the present invention is to provide the complete genome sequence of one group of new Influenza B virus high yield strain.
The object of the present invention is to provide one group of plasmid that includes new Influenza B virus complete genome sequence of the present invention.
Another object of the present invention is to provide one group of primer, be used to amplify whole (8) fragment of Influenza B virus, i.e. the complete genome sequence of Influenza B virus.
Another object of the present invention is to provide a kind of high yield recombinant virus that contains the Influenza B virus antigen property.
Another object of the present invention is to provide a kind of high yield recombinant virus that contains Influenza B virus epidemic strain antigen property.
Another object of the present invention is to provide a kind of by the deactivation of Influenza B virus epidemic strain antigen property and/or the second type influenza virus vaccine that the attenuation recombinant virus is formed of containing of the present invention.
In order to finish purpose of the present invention, the invention provides a kind of new Influenza B virus complete genome sequence, this sequence comprises sequence 1, sequence 2, sequence 3, sequence 4, sequence 5, sequence 6, sequence 7, sequence 8.
These sequence write ups are in sequence table, and wherein sequence 1 is the NS sequence, and sequence 2 is the M sequence, and sequence 3 is the NA sequence, and sequence is 4 HA sequences, and sequence 5 is the Np sequence, and sequence 6 is the Pa sequence, and sequence 7 is the Pb2 sequence, and sequence 8 is the Pb1 sequence.
The present invention also provides one group of plasmid that includes new Influenza B virus complete genome sequence of the present invention.Described plasmid comprises: PCDNA3.1-BPB1, PCDNA3.1-BPB2, PCDNA3.1-BPA, PCDNA3.1-BNP, PCDNA3.1-BHA, PCDNA3.1-BNA, PCDNA3.1-BNS, PCDNA-3.1-BM, PHH21-BPB1, PHH21-BPB2, PHH21-PA, PHH21-NP, PHH21-HA, PHH21-NA, PHH21-NS, PHH21-BM, PIVVII-BNS, PIIVII-BM, PIVVII-BHA, PIVVII-BNA, PIVVII-BNP, PIVVII-BPA, PIVVII-BPB2, PIVVII-BPB1, preferably PIVVII-BNS, PIVVII-BMPIVVII-BHA, PIVVII-BNA, PIVV2II-BNP, PIVVII-BPB1, PIVVII-BPB2, PIVV-BPA.
The present invention also provides one group of primer, is used to amplify 8 fragments of the full sequence 1 of Influenza B virus to sequence 8, i.e. the complete genome sequence of Influenza B virus, and this primer comprises:
BM-NS-1:5’-ATCGTCTCTGGGAGCAGAAGCAGAGCA-3’
BM-NS-2:5’-GGCGTCTCGTATTAGTAGTAACAAGAG-3’
BM-U-1:5’-AACGTCTCTGGGAGCAGAAGC-3’
BM-U-2:5’-GGCGTCTCGTATTAGTAGAAAC-3’
BM-PA-1-:5-TTCGTCTCAGGGAGCAGAAGCGGT-3
BM-PB1-1:5-TTCGTCTCTGGGAGCAGAAGCGGAGCTTTAAG-3
BM-PB2-1:-5-TTGGTCTCAGGGAGCAGAAGCGGAGCGTTTTCAAG.-3
The inventor carries out analogy analysis through to the sequence at the Influenza B virus gene fragment two ends among the GENE BANK, design two cover primers, i.e. and BM-NS-1 and BM-NS-2 and BM-U-1 and BM-U-2 whole 8 gene fragments of influenza virus that increase,
With all 8 fragments of RT-PCR method amplification vRNA, with reference to the terminal conserved sequence complementary of viral RNA sequence as primer.
BM-NS-1:5’-ATCGTCTCTGGGAGCAGAAGCAGAGCA-3’
BM-NS-2:5’-GGCGTCTCGTATTAGTAGTAACAAGAG-3’
BM-U-1:5’-AACGTCTCTGGGAGCAGAAGC-3’
BM-U-2:5’-GGCGTCTCGTATTAGTAGAAAC-3’
More than two cover primers can amplify whole 8 fragments of influenza virus.But,, design primer three the big fragments that increase again respectively so be not easy to distinguish because three fragment lengths of influenza virus RNA polymerase are about 2.3Kb
BM-PA-1-:5-TTCGTCTCAGGGAGCAGAAGCGGT-3
BM-PB1-1:5-TTCGTCTCTGGGAGCAGAAGCGGAGCTTTAAG-3
BM-PB2-1:-5-TTGGTCTCAGGGAGCAGAAGCGGAGCGTTTTCAAG.-3
Primer of the present invention can amplify the full genome of high yield strain by the RT-PCR method, and the gene fragment of most Influenza B viruss that can be applied to increase.
The present invention also provides a kind of high yield recombinant virus that contains the Influenza B virus antigen property, and this virus strain contains above-mentioned nucleotide sequence 1 to sequence 8, and the particular case of its sequence is seen sequence table.
The reorganization Influenza B virus strain that obtains through the inventive method on January 15th, 2003 in China Committee for Culture Collection of Microorganisms's common micro-organisms center preservation, B/ capital section/96/2001, its preserving number is 0880.
The present invention also provides 8 plasmid co-transfection mammalian cells using the Influenza B virus gene, and then obtains the method for recombinant virus.
It is a kind of by the deactivation of popular Influenza B virus antigen property and/or the second type influenza virus vaccine that the attenuation recombinant virus is formed of containing of the present invention that the present invention also provides.
The invention still further relates to a kind of method for preparing new Influenza B virus strain of the present invention, this method may further comprise the steps:
With described primer BM-NS-1, BM-NS-2, BM-U-1, BM-U-2, BM-PA-1, BM-PB1-1, BM-PB2-1 amplify the full genomic fragment of Influenza B virus;
The genomic fragment that obtains is linked to each other with the PIVVII carrier;
With PIVVII plasmid transfection 293T that contains described genomic fragment and the MDCK co-cultured cell that obtains;
The supernatant liquor that contains influenza virus of results transfection.
And, the invention still further relates to a kind of method for preparing the second type influenza virus vaccine, this method may further comprise the steps:
On MDCK, cultivate the virus strain of reprovision; Collect this cell culture supernatant; Centrifugal removal fragment; Ultrafiltration obtains concentrating recombinant virus.Described reprovision virus strain is meant and contains sequence 1 of the present invention, sequence 2, sequence 5, sequence 6, sequence 7, the sequence 3 (NA) of sequence 8 and popular influenza virus strain, sequence 4 (HA).
According to well known to a person skilled in the art method, can be to concentrating recombinant virus district band ultracentrifugation; With the PBS washing, centrifugal again.
The present invention also provides a kind of Influenza B virus strain, it is characterized in that its gene order comprises sequence 1 of the present invention, sequence 2, sequence 5, sequence 6, sequence 7, the HA of sequence 8 and popular Influenza B virus strain, NA sequence.
Influenza vaccines of the present invention are a kind of deactivation of reprovision Influenza B virus strain strain and/or the second type influenza virus vaccine of attenuation.
In fact, according to the present invention, the second type influenza virus strain that the contriver obtains has the characteristic of high yield on mammalian cell, and it can overcome the deficiency of producing vaccine with the chicken embryo.This mammalian cell, particularly mdck cell strain can be used as the clone of production of vaccine, and therefore recombinant virus of the present invention has high using value.
In addition, the sequence of six gene fragments of recombinant strain except that HA and NA fragment has played the keying action of decision high yield characteristics, and the advantage of the strain that the inventor packs out is that the time that produces virus after the transfection is fast, only just can produce a large amount of (8 * 10 at 30 hours
4PFU/ML) virus.
Should be noted that reorganization Influenza B virus strain of the present invention equal high yield on chicken embryo and mammalian cell, be particularly suitable for becoming the maternal plant of production of vaccine.
The present invention also provides a kind of Influenza B virus strain, and its gene order comprises sequence 1 of the present invention, sequence 2, sequence 5, sequence 6, sequence 7, the HA of sequence 8 and popular Influenza B virus strain, NA sequence.
Description of drawings
I.8Kb, Fig. 1 has band with the 2.3Kb place for using the BM-U primer respectively at 1.1Kb, and sequencing result is respectively the M fragment, NP fragment and 3 big fragments.
Fig. 2 uses the result of NS primer amplification at 1.1Kb, 1.5Kb, and there is band at the 1.8Kb place,, sequencing result confirms to be respectively NS, HA, NA fragment.
Fig. 3 is that the result of 3 big segmental primer amplified can see band respectively at the 2.3KB place.
Fig. 4, enzyme cut the NS fragment.
Fig. 5, right 1NA-PIVV2Nco1 enzyme is cut, and right 2HA-PIVV2Hind3 enzyme is cut, a left side 1,2,3, PB2 Sca1 enzyme is cut.
Fig. 6 SCA1 enzyme is cut the M fragment.
Fig. 7, the NDE1 enzyme is cut PB2.
Fig. 8, Pvu2 and HIind3 enzyme are cut PA.
Fig. 9, left 1PB2 (PB1) SCA1 enzyme is cut the Sca1 quantity not sufficient.A left side 2, the 3Nco1 enzyme is cut, NP-PIVV2.The right side 1, the 2Hind3 enzyme is cut HA-PIVV2.
Figure 10 is plasmid construction figure.
Figure 11 is experimental principle figure.
Figure 12 is epidemic isolates and high yield strain reprovision schematic diagram.
Embodiment
The acquisition of embodiment 1 Influenza B virus full gene group
Strain: B/ capital section/96/01 derives from national influenza center, and B/ Sichuan/379/99 and B/HongKong/330/01 derive from U.S. CDC.
RT-PCR: doubling dilution is carried out in strain B/ capital section/96/01 that screens, the inoculation mdck cell, results virus after 72 hours uses Rneasy KIT (Qiagen) to extract viral RNA, is dissolved in the dilution of 30ul water.
The RT-PCR reaction system was 94 ℃ of sex change 3 minutes, and 55 ℃ were extended 1 hour, and reversed transcriptive enzyme provides for Invitrogen company, and the PCR system is 72 ℃ of 420Sec of 50 ℃ of 45Sec of 94 ℃ of 45Sec then, and the PFU enzyme is available from (Promega) company.
The full gene group of amplification B/ capital section/96/01 uses BM-NS-1 BM-NS-2 primer amplification to go out the HA and the NA fragment of epidemic isolates, and the PCR product is connected on the PGEM-T carrier (Promega company).
The result who obtains through method of the present invention is: referring to Fig. 1, with the result of NS primer amplification at 1.1Kb, 1.5Kb, there is band at 1.8Kb place, the sequencing result confirmation is respectively NS, HA, NA fragment.Referring to Fig. 2, for using the BM-U primer, I.8Kb band is arranged with the 2.3Kb place respectively at 1.1Kb, sequencing result is respectively the M fragment, NP fragment and 3 big fragments.Referring to Fig. 3, be that the result of 3 big segmental primer amplified can see band respectively at the 2.3KB place.Its sequencing result is seen sequence table.
This shows several groups of primers that adopt the present invention's design, be cloned into Influenza B virus B/
Whole 8 the complete gene fragments of capital section/96/01 strain, and be cloned on the PGEM-T carrier, use fluorescent marker method and measured all
cDna sequence dna.Thereby obtain following 8 gene fragments.
The non-coding region of the Influenza B virus that the present invention obtains and and clip size
The reverse conserved regions of gene forward conserved regions
Size
PB1 BM-PB1-1 BM-PB12397
AGCAGAAGCGGAGCTTTAAG AGTAGAAACACG
PB2 BM-PB2-2381 BM-PB2-2381
AGCAGAAGCGGAGCGTTTTC AGTAGAAACACG
PA BM-PA-1 BM-PB2-2381
2309
AGCAGAAGCGGTGCGTTTG AGTAGAAACACG
1885
AGCAGAAGCAGA(GTT) AGTAGTAACAAG
NP BM-NS-1 BM-NP-1844
1844
AGCAGAAGCAGA(ACA) AGTAGAAACAGC
BM-NS-1 BM-NS-1099
1559
AGCAGAAGCAGA(GCC) AGTAGTAACAAG
M BM-M-1 BM-M-1191
1191
AGCAGAAGCAGGC(ACGG) AGTAGAAACAAC
NS BM-NS-1 BM-NS-1099
1099
AGCAGAAGCAGA AGTAGTAACAAG
In the present invention, used 8 pUC pUCs, preferred plasmid is respectively PIVVII-BPB1, PIVVII-BNS, PIVVII-BM, PIVVII-BHA, PIVVII-BNA, PIVVII-BNP, PIVVII-BPB2, pack out a strain Influenza B virus behind the PIVVII-BPA cotransfection mammalian cell, and the strain of packing out has been carried out the virulence detection, obtained the virus strain of equal high yield on mammalian cell and chicken embryo.
The structure of embodiment 2 PIVVII plasmids
One: the structure of PIVVII plasmid:
Referring to plasmid figure and the experimental principle shown in Figure 10 and Figure 11.
The characteristics of 1:PIVVII plasmid: the contriver has made up the PIVVII plasmid.The characteristics of this plasmid are promotor and the terminator sequences that has polysaccharase I and polymerase II simultaneously, and the promotor direction of polysaccharase I and polymerase II is opposite.Viral genome is inserted between the BSMB1 site of the promotor of polysaccharase 1 and terminator sequence, under the effect of polysaccharase 1 promotor, transcribe out the genome of virus, under the effect of polymerase II promotor, transcribe out the mRNA of virus, translate the albumen of virus
The construction process of 2:PIVVII plasmid:, use primer with the promotor and the terminator sequence amplification of PHH21 plasmid (Neumann G present):
Upstream: 5 ' ATCCCTAGGGCGGCCGGGAGGGCGTCCCCGGCC3 '
Downstream: 5 ' GTGAAGCTTCGGAGTACCGGTCGACCTCCGAAG3 '
After using AvuII and HindHI double digestion then, be connected to P
cOn the DNA3.1, confirm that through order-checking the sequence of inserting is a target sequence then.
Embodiment 3 virus genomic fragments link to each other with the PIVVII carrier respectively
PIVVII plasmid vector BSMB1 linearization for enzyme restriction with embodiment 2 obtains reclaims the PIVVII fragment that test kit reclaims linearization with Qiagen then.Equally, the target fragment that is connected to the PGEM-T carrier is cut with the BSMB1 enzyme, then, reclaim target fragment.The described fragment of sequence 1-8 is connected respectively on the PIVVII carrier, and system is the 3ul target fragment, 1ul carrier, 1ulT
4Dna ligase (Promega) 15ulddH
2O, thus obtain connecting product P IVVII-BX.
Embodiment 4 transforms
The connection product that embodiment 3 is obtained is transformed in the competence bacteria (Sure bacterium), 42 ℃ of heat-shockeds 60 seconds, ice bath 5 minutes, again 37 ℃ of concussions 45 minutes, centrifugal, get precipitation and be coated with flat board, spend the night in 37 ℃ of incubators, choose single colony inoculation next day in the 5mlLB substratum, little upgrading grain after 37 ℃ of concussions are spent the night.
Embodiment 5 enzymes are cut evaluation
With well known to a person skilled in the art method accordingly restriction endonuclease is identified whether target sequence links to each other with carrier.PIVVII-BNS Nde1 Pst1 double digestion wherein, clip size is 1.1Kb 3.5Kb 1.5Kb.
PIVVII-BNP Nco1 enzyme is cut, 500bp 700bp 900bp 1.8Kb.
PIVVII-BM Sca1 enzyme is cut, and clip size is 500bp 300bp 1.1Kb 1.7Kb 3.4Kb.
PIVVII-BHA Nco1 enzyme is cut, and clip size is 1.7Kb 1.5Kb 700bp.
PIVVII-BNA Nco1 enzyme is cut, and clip size is 1.6Kb (2) 700bp.
PIVVII-BPB2 Nde1 enzyme is cut, and clip size is 1.3Kb 900bp 6.7Kb.
PIVVII-BPB1 Nde1 enzyme is cut, and clip size is 500bp, 700bp, 900bp, 1.5Kb, 3.7Kb.
PIVVII PA enzyme is cut, and clip size is 1.0Kb, 1.6Kb, 4.7Kb.
Wherein: the result that enzyme is cut is: referring to following each the description of the drawings.
Fig. 4, enzyme cut the NS fragment.
Fig. 5, right 1NA-PIVV2Nco1 enzyme is cut, and right 2HA-PIVV2Hind3 enzyme is cut, a left side 1,2,3, PB2 Sca1 enzyme is cut.
Fig. 6 SCA1 enzyme is cut the M fragment.
Fig. 7, the NDE1 enzyme is cut PB2.
Fig. 8, Pvu2 and HIind3 enzyme are cut PA.
Fig. 9, left 1PB2 (PB1) SCA1 enzyme is cut the Sca1 quantity not sufficient.A left side 2, the 3Nco1 enzyme is cut, NP-PIVV2.The right side 1, the 2Hind3 enzyme is cut HA-PIVV2.
Embodiment 6 transfections
293T and mdck cell are cultivated altogether at 12.5CM
2Tissue Culture Flask in treat that cell 80% in flakes after, 1ug/DNA Per and 2ulLF2000 are blended in room temperature placement 45 minutes, join then in the cell bottle, after 6 hours, keeping liquid with optim-MEM continues to hatch in 33 ℃ of incubators, add TPCK-Trypsin to final concentration 1ug/ml behind 30 hours of transfection, gathered in the crops respectively 24 hours, the viral suspension of 48 hours and 72 hours is inoculated mdck cell.
The continuous passage of embodiment 7 recombinant viruses
The inoculation recombinant virus the day before yesterday with cell inoculation in culturing bottle, second angel's cell count reaches 3-4 * 10
6, the MOI value of virus inoculation is 1 * 10
-4TCID50/, 1 * 10
-5The every cell of CID50/ is kept liquid and is comprised TPCK-Trypsin, adds respectively at metainfective 24,48 hours to make the final concentration of TPCK-Trypsin reach 1ug/ml again, cultivates 72 or 96 hours results virus at 33 ℃.
The detection of embodiment 8 recombinant virus output
Recombinant virus is inoculated the first-generation behind the mdck cell, and in the 5th generation, in the tenth generation and the 15 generation, done the detection of TCID50 and PFU respectively.
TCID50 detects: cell is cultivated into individual layer on 24 orifice plates, virus is carried out doubling dilution, inoculating cell is to 24 orifice plates, 4 holes of the parallel adding of each extent of dilution, every hole adds 200UL, hatches after 1 hour for 33 ℃ and uses HANK ' S to wash, and adds the liquid of keeping that comprises TPCK-Trypsin then.Added TPCK-Trypsin respectively at metainfective 24,48,72 hours, frozen in metainfective 72 hours results virus in-70 ℃ of refrigerator overnight, calculated TCID50 according to HAU in second day.
PFU detects: virus is carried out doubling dilution, be inoculated in little square vase, every little square vase adds 500UL viral dilution liquid, 33 ℃ hatch 1 hour after, with the flushing of HANKS liquid, add the first layer covering liquid then, hatch adding second layer covering liquid after 72 hours, count plaque after 24 hours for 33 ℃.
Order-checking: the metainfective first-generation and the 15 generation viral suspension extraction viral RNA are measured the segmental dna sequence dna of HA.
The result shows the feature of recombinant virus: use reverse genetics with 8 plasmid co-transfection eukaryotic cells after, obtained recombinant virus, strain for high yield on mdck cell, at the also very high evidence of output on the chicken embryo be: recombinant virus goes down to posterity on the chicken embryo, wherein the HAU that the suspension of 24 hours supernatants inoculation mdck cells after 1 generation inoculates the chicken embryo after the transfection is up to 1280, uploads for 15 generations at mdck cell.First-generation HAU is 1: 40 to the 15th generation 1: 640 on mdck cell, and the titre of infective virus is from 8 * 10 of the first-generation
4PFU, 6.5Log
10 TCID50To 2 * 10 of the 15 generation
9PFU, 8.5Log
10 TCID50, the virulence of virus has the trend of increase after 15 generations as can be seen, and high yield characteristics is maintained and improves.HA is checked order after the sequence of the HA of the sequence of the HA of comparison the 15th generation virus and 24 hours results virus of transfection is in full accord.
Embodiment 9 makes up the second type influenza virus recombinant virus that contains the epidemic isolates antigen property
Referring to Figure 12, the HA of epidemic isolates, remaining sequence 1 of the present invention of NA fragment and high yield strain, sequence 2, sequence 5, sequence 6, sequence 7, mammalian cell such as 6 fragment cotransfections such as sequence 8 grades can obtain reprovision virus as vaccine strain.
Make up recombinant virus (the Eight-plasmid system for rapid generation of influenza virus vaccines.Vaccine.2002 Aug 19 that contains the epidemic isolates antigen property with reference to the method that well known to a person skilled in the art; 20 (25-26): 3165-70.).
In other words, experimental technique is with embodiment 6, and different is with V system is the HA of B/HongKong/330/01 B/ Sichuan/379/99 and the PB2 of NA fragment and B/ capital section/96/01 with Y, PB1, PA, M, NS, NP reprovision, produce the reprovision virus of 6+2, behind transfection mdck cell and the inoculated into chick embryo, still keep the characteristic of high yield, consequent reprovision virus can be used as vaccine strain.
Embodiment 10 preparation second type influenza virus vaccines
On Rotary Machine, cultivate the mdck cell of the virus strain that contains reprovision; 33 degrees centigrade of culture temperature 72-96 hour, are collected this cell culture supernatant then; Centrifugal 12000-15000RPM removes fragment; Ultrafiltration obtains concentrating recombinant virus, and wherein said reprovision virus strain is meant and contains sequence 1 of the present invention, sequence 2, sequence 5, sequence 6, sequence 7, the HA of sequence 8 and popular influenza virus strain, NA sequence.
To the virus that obtains adopt well known to a person skilled in the art the method deactivation after, add suitable adjuvant and make operable Influenza B virus vaccine.
Sequence table
<110〉CDC virus disease control institute
<120〉reorganization Influenza B virus strain of high yield and uses thereof
<130>
<160>8
<170>PatentIn?version?3.1
<210>1
<211>1099
<212>DNA
<213〉Influenza B virus (influenza B virus)
<400>1
agcagaagca?gagcatttgt?ttagtcactg?gcaaacgaaa?aaatggagga?caacatgatc 60
acaacacaaa?ttgaggtggg?tccgggagca?accaatgcca?ccataaactt?tgaagcagga 120
attttggagt?gctatgaaag?gctttcatgg?caaagagccc?ttgactaccc?tggtcaagac 180
cgcctaaaca?ggctaaagag?aaaattggaa?tcaagaataa?agactcacaa?caaaagtgag 240
cctgaaagta?aaaggatgtc?tcttgaagag?agaaaagcta?ttggggtaaa?aatgatgaaa 300
gtgctcctat?ttatgaaccc?atctgctgga?gttgaagggt?ttgagccata?ttgtacgaaa 360
aatccctcca?atagcaactg?tccgaactgc?aattggtctg?attaccctcc?aacaccagga 420
aagtaccttg?atgacataga?agaagaagaa?ccggagaatg?ttggtgaccc?aactgaaata 480
gtattaaggg?acatgaacaa?cagagatgca?aggcaaaaga?taaaagagga?agtaaacact 540
cagaaagaag?ggaaattccg?tttaacgata?aaaagggata?tacgtaatgt?gttgtccttg 600
agagtgttgg?taaacggaac?attcatcaag?caccctaatg?gatacaagtc?cttatcaact 660
ctgcatagat?tgaatgcata?tgaccagagt?ggaagacttg?ttgctaaact?tgttgctact 720
gatgatctta?cagtggagga?tgaagaagat?ggccatcgga?tcctcaactc?actcttcgag 780
cgttttaatg?aaggacattc?aaagccaatt?cgagcagctg?aaactgcggt?gggagtctta 840
tcccaatttg?gtcaagagca?ccgattatca?ccagaagaga?gagacaatta?gactggttac 900
ggaagaactt?tatcttttaa?gtaaaagaat?tgatgataac?atattgttcc?acaaaacagt 960
aatagccaac?agctccataa?tagctgacat?gattgtatca?ttatcattat?tggaaacatt 1020
gtatgaaatg?aaggatgtgg?ttgaagtgta?cagcaggcag?tgcttgtgaa?tttaaaataa 1080
aaatcctctt?gttactact 1099
<210>2
<211>1190
<212>DNA
<213〉Influenza B virus (influenza B virus)
<400>2
agcagaagca?ggcactttct?taaaatgtcg?ctgtttggag?acacaattgc?ctacctgctt 60
tcattgacag?aagatggaga?aggcaaagca?gaactagcag?aaaaattaca?ctgttggttc 120
ggtgggaaag?aatttgacct?agactctgcc?ttggaatgga?taaaaaacaa?aagatgctta 180
actgatatac?agaaagcact?aattggtgcc?tctatctgct?ttttaaaacc?caaagaccag 240
gaaagaaaaa?gaagattcat?cacagagccc?ctatcaggaa?tgggaacaac?agcaacaaaa 300
aagaagggcc?tgattctagc?tgagagaaaa?atgagaagat?gtgtgagctt?ccatgaagca 360
tttgaaatag?cagaaggcca?tgaaagctca?gcgttactat?attgtctcat?ggtcatgtac 420
ctgaatcctg?gaaattattc?aatgcaagta?aaactaggaa?cgctctgtgc?tttgtgcgaa 480
aaacaagcat?cacattcaca?cagggctcat?agcagagcag?cgagatcttc?agtgcccgga 540
gtgagacgag?aaatgcagat?ggtctcagct?atgaacacag?caaaaacaat?gaatggaatg 600
ggaaaaggag?aagacgtcca?aaaactggca?gaagagctgc?aaagcaacat?tggagtattg 660
agatctcttg?gggcaagtca?aaagaatggg?gaaggaattg?caaaggatgt?aatggaagtg 720
ctaaagcaga?gctctatggg?aaattcagct?cttgtgaaga?aatacctata?atgctcgaac 780
catttcagat?tctttcaatt?tgttctttta?ttttatcagc?tctccatttc?atggcttgga 840
caataggaca?tttgaatcaa?ataaaaagag?gagtaaacat?gaaaatacga?ataaagggac 900
caaataaaga?gacaataaac?agagaggtat?caattttgag?acacagttac?caaaaagaaa 960
tccaggccaa?agaaacaatg?aaggaagtac?tctctgacaa?catggaggta?ttgagtgacc 1020
acatagtaat?tgaggggctt?tctgctgaag?agataataaa?aatgggtgaa?acagttttgg 1080
aggtagaaga?attgcattaa?attcaatttt?tactgtactt?cttactatgc?atttaagcaa 1140
attgtaatca?atgtcagcaa?ataaactgga?aaaagtgcgt?tgtttctact 1190
<210>3
<211>1558
<212>DNA
<213〉Influenza B virus (influenza B virus)
<400>3
agcagaagca?gagcatcttc?tcaaaaactg?aggcaaatag?gccaaaaatg?aacaatgcta 60
ccttcaacta?tacaaacgtt?aaccctattt?ctcacatcag?ggggagtgtt?attatcacta 120
tatgtgtcag?cttcactgtc?atacttacta?tattcggata?tattgctaaa?attttcacaa 180
acagaaataa?ctgcaccaac?aatgccattg?gattgtgcaa?acgcatcaaa?tgttcaggct 240
gtgaaccgtt?ctgcaacaaa?aggagtgaca?cttcttcccc?cagaaccgga?gtggacgtac 300
cctcgtttat?cttgcccggg?ctcaaccttt?cagaaagcac?tcctaattag?ccctcataga 360
ttcggagaaa?ccaaaggaaa?ctcagctccc?ttgataataa?gggaaccttt?tattgcttgt 420
ggaccaaagg?aatgcaaaca?ctttgctcta?acccattatg?cagctcaacc?agggggatac 480
tacaatggaa?caagagaaga?cagaaacaag?ctgaggcatc?taatttcagt?caaattgggc 540
aaaatcccaa?cagtagaaaa?ctctattttc?cacatggcag?cttggagcgg?gtccgcatgc 600
catgatggta?gagaatggac?atatatcgga?gttgatggcc?ctgacagtaa?tgcattgctc 660
aaaataaaat?atggagaagc?atatactgac?acataccatt?cctatgcaaa?aaacatccta 720
aggacacaag?aaagtgcctg?caattgcatc?gggggagatt?gttatcttat?gataactgat 780
ggctcagctt?cagggattag?tgaatgcaga?ttccttaaga?ttcgagaggg?ccgaataata 840
aaagaaatat?ttccaacagg?aagagtaaaa?catactgaag?aatgcacatg?cggatttgcc 900
agcaataaaa?ccatagaatg?tgcctgtaga?gataacagtt?acacagcaaa?aagacccttt 960
gtcaaattaa?atgtggagac?tgatacagcg?gaaataagat?tgatgtgcac?agagacttat 1020
ttagacaccc?ccagaccaga?tgatggaagc?ataacagggc?cttgcgaatc?taatgggaac 1080
aaagggagtg?gaggcatcaa?gggaggattt?gttcatcaaa?gaatggcatc?caagattgga 1140
aggtggtact?ctcgaacgat?gtctaaaact?aaaagaatgg?ggatgggact?gtatgtcaag 1200
tatgatggag?acccatggac?tgacagtgaa?gcccttgctc?ttagtggagt?aatggtttca 1260
atggaagaac?ctggttggta?ttcctttggc?ttcgaaataa?aagataagaa?atgtgatgtc 1320
ccctgtattg?ggatagaaat?ggtacatgat?ggtgggaaaa?cgacttggca?ctcagcagca 1380
acagccattt?actgtttaat?gggctcagga?caactactgt?gggacactgt?cacaggtgtt 1440
gatatggctc?tgtaatggag?gaatggttga?gtctgttcta?aaccctttgt?tcctattttg 1500
tttgaacaat?tgtccttact?gaacttaatt?gtttctgaaa?aatgctcttg?ttactact 1558
<210>4
<211>1882
<212>DNA
<213〉Influenza B virus (influenza B virus)
<400>4
agcagaagca?gagcattttc?taatatccac?aaaatgaagg?caataattgt?actactcatg 60
gtagtaacat?ccaatgcaga?tcgaatctgc?actgggataa?catcttcaaa?ctcacctcat 120
gtggtcaaaa?cagctactca?aggggaggtc?aatgtgactg?gtgtgatacc?actgacaaca 180
acaccaacaa?aatctcattt?tgcaaatctc?aaaggaacaa?ggaccagagg?gaaactatgc 240
ccagactgtc?tcaactgcac?agatctggat?gtggccttgg?gcagaccaat?gtgtgtgggg 300
accacacctt?cggcaaaagc?ttcaatactc?cacgaagtca?gacctgttac?atccgggtgc 360
tttcctataa?tgcacgacag?aacaaaaatc?agacaactac?ccaatcttct?cagaggatat 420
gaaaatatca?ggttatcaac?ccaaaacgtt?atcgatgcag?aaaaggcacc?aggaggaccc 480
tacagacttg?gaacctcagg?atcttgccct?aacgctacca?gtaaaagcgg?atttttcgca 540
acaatggctt?gggctgtccc?aaaggacaac?aacaaaaatg?caacgaaccc?actaacagta 600
gaagtaccac?acgtttgtac?agaaggggaa?gaccaaatta?ctgtttgggg?gttccattca 660
gataacaaaa?ctcaaatgaa?aaacctctat?ggagactcaa?atcctcaaaa?gttcacctca 720
tctgctaatg?gagtaaccac?acattatgtt?tctcagattg?gcggcttccc?agatcaaaca 780
gaagacggag?gactaccaca?aagcggcaga?attgttgttg?attacatggt?gcaaaaacct 840
gggaaaacag?gaacaattgt?ctatcaaaga?ggtgttttgt?tgcctcaaaa?ggtgtggtgc 900
gcgagtggca?ggagcaaagt?aataaaaggg?tccttgcctt?taattggtga?agcagattgc 960
cttcatgaaa?aatacggtgg?attaaacaaa?agcaagcctt?actacacagg?agaacatgca 1020
aaagccatag?gaaattgccc?aatatgggtg?aaaacacctt?tgaagcttgc?caatggaacc 1080
aaatatagac?ctcctgcaaa?actattaaag?gaaaggggtt?tcttcggagc?tattgctggt 1140
ttcctagaag?gaggatggga?aggaatgatt?gcaggttggc?acggatacac?atctcacgga 1200
gcacatggag?tggcagtggc?ggcagacctt?aagagtacgc?aagaagctat?aaacaagata 1260
acaaaaaatc?tcaattcttt?gagtgagcta?gaagtaaaga?atcttcaaag?actaagtggt 1320
gccatggatg?aactccacaa?cgaaatactc?gagctggatg?agaaagtgga?tgatctcaga 1380
gctgacacta?taagctcgca?aatagaactt?gcagtcttgc?tttccaacga?aggaataata 1440
aacagtgaag?atgagcatct?attggcactt?gagagaaaac?taaagaaaat?gctgggtccc 1500
tctgctgtag?acataggaaa?tggatgcttc?gaaaccaaac?acaagtgcaa?ccagacctgc 1560
ttagacagga?tagctgctgg?cacctttaat?gcaggagaat?tttctctccc?cacttttgat 1620
tcactgaaca?ttactgctgc?atctttaaat?gatgatggat?tggataacca?tactatactg 1680
ctctattact?caactgctgc?ttctagtttg?gctgtaacat?tgatgctagc?tatttttatt 1740
gtttatatgg?tctccagaga?caacgtttca?tgctccatct?gtctataagg?aagattaagc 1800
cttgtatttt?cctttattgc?agtgcttgtt?tgcttgtcat?cattacaaag?aaacgttatt 1860
gaaaaatgct?cttgttacta?ct 1882
<210>5
<211>1844
<212>DNA
<213〉Influenza B virus (influenza B virus)
<400>5
agcagaagca?cagcattttc?ttgtgaactt?caagcaccaa?taaaagaact?gaaaatcaaa 60
atgtccaaca?tggatattga?cggtatcaac?actgggacaa?ttgacaaaac?accggaggaa 120
ataacttctg?gaaccagtgg?gacaaccaga?ccaatcatca?gaccagcaac?ccttgcccca 180
ccaagcaaca?aacgaacccg?gaacccatcc?ccggaaagag?caaccacaag?cagtgaagct 240
gatgtcggaa?ggaaaaccca?aaagaaacag?accccgacag?agataaagaa?gagcgtctac 300
aatatggtag?tgaaactggg?cgaattctat?aaccagatga?tggttaaagc?tggactcaac 360
gatgacatgg?agagaaatct?aatccaaaat?gcgcatgctg?tggaaagaat?tctattggct 420
gccactgatg?acaagaaaac?tgaattccag?aagaaaagaa?atgccagaga?tgtcaaagaa 480
gggaaagaag?aaatagacca?caacaaaaca?ggaggcacct?tttacaagat?ggtaagagat 540
gataaaacca?tctacttcag?ccctataaga?attacctttt?taaaagaaga?ggtgaaaaca 600
atgtacaaaa?ccaccatggg?gagtgatggc?ttcagtggac?taaatcacat?aatgattggg 660
cattcacaga?tgaatgatgt?ctgtttccaa?agatcaaagg?cactaaaaag?agttggactt 720
gacccttcat?taatcagtac?ctttgcagga?agcacaatcc?ccagaagatc?aggtgcaact 780
ggtgttgcga?tcaaaggagg?tggaacttta?gtggctgaag?ccattcgatt?tataggaaga 840
gcaatggcag?acagaggact?attgagagac?atcaaagcca?agactgccta?tgaaaagatt 900
cttctgaatc?taaaaaacaa?atgctctgcg?ccccaacaaa?aggctctagt?tgatcaagtg 960
atcggaagta?gaaatccagg?gattgcagac?attgaagatc?taaccctgct?tgctcgtagt 1020
atggtcgttg?ttaggccctc?tgtggcgagc?aaagtagtgc?ttcccataag?catttacgcc 1080
aaaatacctc?aactagggtt?caatgttgaa?gagtactcca?tggttggcta?cgaagccatg 1140
gctctttaca?atatggcaac?acctgtttcc?atattaagaa?tgggggatga?tgcaaaagat 1200
aaatcgcaat?tattcttcat?gtcttgcttc?ggggctgcct?atgaagacct?gagagttttg 1260
tctgcattaa?caggcacaga?attcaagcct?agatcagcat?taaaatgcaa?gggtttccat 1320
gttccagcaa?aggaacaggt?ggaaggaatg?ggggcagctc?tgatgtccat?caagctccag 1380
ttttgggctc?caatgaccag?atctggggga?aacgaagtag?gtggagacgg?agggtctggc 1440
caaataagtt?gcagcccagt?gtttgcagtg?gaaagaccta?ttgctctaag?caagcaagtt 1500
gtaagaagaa?tgctgtcgat?gaatattgag?ggacgtgatg?cagatgtcaa?aggaaatcta 1560
ctcaagatga?tgaatgactc?aatggctaag?aaaaccagtg?gaaatgcttt?cattgggaag 1620
aaaatgtttc?aaatatcaga?caaaaacaaa?accaatccag?ttgaaattcc?aattaagcag 1680
accatcccca?atttcttctt?tgggagggac?acagcagagg?attacgatga?cctcgattat 1740
taaagcaaca?aaatagacac?tatgactgtg?attgtttcaa?tacgtttgga?atgtgggtgt 1800
ttactcttat?taaaataaat?ataaaaaatg?ctgttgtttc?tact 1844
<210>6
<211>2305
<212>DNA
<213〉Influenza B virus (influenza B virus)
<400>6
agcagaagcg?gtgcgtttga?tttgccataa?tggatacttt?tatcacaaga?aacttccaga 60
ctacaataat?acaaaaggcc?aaaaacacaa?tggcagaatt?tagtgaagat?cctgaactac 120
aaccagcaat?gctattcaac?atctgcgtcc?atctagaggt?ttgctatgta?ataagtgaca 180
tgaatttcct?tgatgaagaa?ggaaaagcat?atacagcatt?agaaggacaa?gggaaagaac 240
aaaacttgag?accacaatat?gaagtaattg?agggaatgcc?aagaactata?gcatggatgg 300
tccaaagatc?cttagctcaa?gagcatggaa?tagagactcc?aaagtatctg?gctgatttgt 360
ttgattataa?aaccaagaga?tttatagaag?tcggaataac?aaaaggattg?gctgatgatt 420
acttttggaa?aaagaaagaa?aaactgggaa?atagcatgga?actgatgata?ttcagctaca 480
atcaagacta?ttcgttaagt?aatgaatcct?cattggatga?ggaagggaaa?gggagagtgc 540
taagcagact?cacagaactt?caggccgaat?taagtctaaa?aaacctatgg?caagttctca 600
taggagaaga?agatgttgaa?aagggaattg?actttaaact?tggacaaaca?atatctagac 660
taagggatat?atctgttcca?gctggtttct?ccaattttga?aggaatgagg?agctacatag 720
acaatataga?tcctaaagga?gcaatagaga?gaaatctagc?aaggatgtct?cccttagtat 780
cagccacacc?taaaaagttg?aaatgggagg?acctaagacc?aatagggcct?cacatttaca 840
accatgagct?accagaagtt?ccatacaatg?cctttcttct?aatgtctgat?gaattggggc 900
tggccaatat?gactgaggga?aggtccaaaa?aaccgaagac?attagccaaa?gaatgtctag 960
aaaagtactc?aacactaagg?gatcaaactg?acccaatatt?aataatgaaa?agcgaaaaag 1020
ctaacgaaaa?tttcctatgg?aaactttgga?gggactgtgt?aaatacaata?agtaatgagg 1080
aaatgagtaa?cgagttacag?aaaaccaatt?atgccaaatg?ggccacaggg?gatggattga 1140
cataccagaa?aataatgaaa?gaagtagcaa?tagacgacga?aacaatgtgc?caagaagagc 1200
ctaaaatccc?taacaaatgt?agagtggcag?cttgggttca?aacagagatg?aatctattga 1260
gcactctgac?aagtaaaaga?gctctggact?tgccagaaat?agggccagac?gtggcccccg 1320
tggagcatat?agggagtgaa?agaaggaaat?actttgttaa?tgaaatcaac?tattgtaagg 1380
cctctacagt?tatgatgaag?tatgtgcttt?tccacacttc?attattgaat?gaaagcaatg 1440
ccagcatggg?aaagtacaaa?gtaataccaa?taaccaatag?agtagtaaat?gaaaaaggag 1500
aaagtttcga?catgctttat?ggtctggcgg?ttaaaggaca?atctcatctg?aggggagata 1560
ctgatgtcgt?aacagttgta?actttcgaat?ttagtagtac?agatcccaga?gtggactcag 1620
gaaagtggcc?aaaatatact?gtgtttagga?ttggctccct?atttgtgagt?gggagggaaa 1680
aatctgtgta?cctatattgc?cgagtaaatg?gcacaaataa?gatccaaatg?aaatggggaa 1740
tggaagctag?aagatgtctg?cttcaatcaa?tgcaacaaat?ggaagcaatt?gttgaacaag 1800
aatcatcggt?acaaggatat?gacatgacca?aagcttgttt?caagggagac?agaataaata 1860
gccccaaaac?tttcagtatt?gggactcaag?aaggaaaact?agtaaaagga?tcctttggaa 1920
aagcactaag?agtaatattt?actaaatgtt?tgatgcacta?tgtatttgga?aatgcccaat 1980
tggaggggtt?tagtgccgag?tctagaagac?ttctactgtt?gattcaagca?ttaaaggaca 2040
gaaagggccc?ttgggtgttc?gacttagagg?gaatgtattc?tggaatagaa?gaatgtatta 2100
gtaacaaccc?ttgggtaata?cagagtgcat?actggttcaa?tgaatggttg?ggctttgaaa 2160
aggaggggag?taaagtatta?gaatcagtag?atgaaataat?ggatgaataa?aaggacatag 2220
tactcaattt?agtactattt?tgttcattat?gtatctaaac?atccaataaa?aagaatcaag 2280
aatcaaaaat?gcacgtgttt?ctact 2305
<210>7
<211>2397
<212>DNA
<213〉Influenza B virus (influenza B virus)
<400>7
agcagaagcg?gagcgttttc?aagatgacat?tggctaaaat?tgaattgtta?aaacaactgt 60
taagggacaa?tgaagccaaa?acagtattga?aacaaacaac?ggtagaccaa?tacaacataa 120
taagaaaatt?caatacatca?agaattgaaa?agaatccttc?attaaggatg?aagtgggcaa 180
tgtgttccaa?ttttcccttg?gctctgacca?agggtgacat?ggcaaacaga?atccccttgg 240
aatacaaggg?aatacaactt?aaaacaaatg?ctgaagacat?aggaactaaa?ggccaaatgt 300
gctcaatagc?agcagttacc?tggtggaata?catatggacc?aataggagat?actgaaggtt 360
ttgaaaaggt?ctatgaaagc?tttttcctca?gaaagatgag?acttgacaat?gccacttggg 420
gccgaataac?ttttggccca?gttgaaagag?taagaaaaag?ggtactgcta?aaccctctaa 480
ccaaggaaat?gcctccagat?gaagcaagta?atgtgataat?ggaaatattg?ttccctaagg 540
aagcaggaat?accaagagaa?tctacttgga?tacataggga?actgataaaa?gaaaaaagag 600
aaaaattgaa?aggaacgatg?ataactccca?ttgtactggc?atacatgctt?gagagggaat 660
tggttgccag?aagaaggttc?ctgccggtgg?caggagcaac?atcagctgag?ttcatagaaa 720
tgctacactg?cttacaaggt?gaaaattgga?gacaaatata?tcacccagga?gggaataaac 780
ttactgaatc?taggtctcaa?ttgatgattg?tggcttgtag?aaagataatc?agaagatcaa 840
tagtcgcatc?aaacccattg?gagctagctg?tggaaattgc?aaacaagact?gtaatagata 900
ctgaaccttt?gaaatcatgt?ctgacagcca?tagacggagg?tgatgtagcc?tgtgacataa 960
taagagctgc?attagggcta?aagatcagac?aaagacaaag?atttggacga?cttgaactaa 1020
agagaatatc?aggaagagga?ttcaaaaatg?atgaagaaat?attaatcgga?aacggaacaa 1080
tacagaagat?tggaatatgg?gacggagaag?aggagttcca?tgtaagatgt?ggtgaatgca 1140
ggggaatatt?aaaaaagagc?aaaatgagaa?tggaaaaact?actgataaat?tcagctaaaa 1200
aggaggacat?gaaagattta?ataatcttgt?gcatggtatt?ttctcaagac?actaggatgt 1260
tccaaggagt?gaggggagaa?ataaattttc?ttaatagagc?aggccaactt?ttatctccaa 1320
tgtaccaact?ccaaagatat?tttttgaaca?gaagtaacga?tctctttgat?caatgggggt 1380
atgaggaatc?acccaaagca?agcgagctac?atgggataaa?tgaattaatg?aatgcatctg 1440
actacacttt?gaaaggggtt?gtagtaacaa?aaaatgtgat?tgatgatttt?agttctactg 1500
aaacagaaaa?agtatctata?acaaaaaatc?ttagtttgat?aaaaaggact?ggggaagtca 1560
taatgggggc?caatgacgta?agtgaattag?aatcacaagc?tcagctaatg?ataacatatg 1620
atacacctaa?gatgtgggag?atgggaacaa?ccaaagaact?ggtgcaaaac?acctatcaat 1680
gggtgctaaa?aaatttggta?acactgaagg?ctcagtttct?tctaggaaaa?gaagacatgt 1740
tccaatggga?tgcatttgaa?gcatttgaaa?gcataattcc?ccagaaaatg?gctggccagt 1800
acagtggatt?tgcaagagca?gtgctcaaac?aaatgagaga?ccaagaggtc?atgaaaactg 1860
accagttcat?aaagttgttg?cccttttgtt?tctcaccacc?aaaattaagg?agcaatgggg 1920
agccttatca?gtttttgagg?cttgtattga?agggaggagg?agaaaatttc?atcgaagtaa 1980
ggaaagggtc?tcctctattc?tcttacaatc?cacaaacaga?agtcctaact?atatgcggca 2040
gaatgatgtc?attaaaggga?aaaattgaag?atgaagaaag?aaatagatca?atggggaatg 2100
cagtactggc?gggctttctt?gttagtggca?agtatgaccc?ggatcttgga?gatttcaaaa 2160
ctattgaaga?acttgaaaag?ctaaaaccgg?gggagaaagc?aaacatctta?ctttatcaag 2220
gaaaacccgt?taaagtagtt?aaaaggaaaa?gatatagtgc?tttatccaat?gacatttcac 2280
agggaattaa?gagacaaaga?atgacagttg?agtccatggg?gtgggccttg?agctaatata 2340
aatttatcca?ttaattcaat?aaacacaatt?gattgaaaaa?atgctcgtgt?ttctact 2397
<210>8
<211>2369
<212>DNA
<213〉Influenza B virus (influenza B virus)
<400>8
agcagaagcg?gagcttttaa?gatgaatata?aatccttatt?ttctcttcat?agatgtaccc 60
atacaggcag?caatttcaac?aacattccca?tacaccggtg?ttccccctta?ttcccatgga 120
acgggaacag?gccacacaat?agacaccgtg?atcagaacac?atgagtactc?gaacaaggga 180
aaacaatatg?tttctgacat?cacaggatgt?acaatggtag?atccaacaaa?tggaccatta 240
cccgaagaca?atgagccaag?tgcctatgca?caattagatt?gcgttctgga?ggctttggat 300
agaatggatg?aggaacatcc?aggtctgttt?caggcagcct?cacagaatgc?catggaggca 360
ctaatggtca?caactgtaga?caaattgacc?caggggagac?agacttttga?ttggacagta 420
tgtagaaacc?agcctgctgc?aacggcacta?aacacaacaa?taacctcctt?taggttgaat 480
gatttgaatg?gagctgacaa?gggtggattg?gtaccctttt?gccaagatat?cattgattca 540
ttggacaagc?ctgaaatgac?tttcttctca?gtaaagaata?taaagaaaaa?gttgcctgca 600
aaaaacagaa?agggtttcct?cataaagaga?ataccaatga?aagtaaaaga?caggatatcc 660
agagtggaat?acatcaaaag?agcattgtca?ttaaacacaa?tgacaaaaga?tgctgaaagg 720
ggcaaactaa?aaagaagagc?gattgcaacc?gctgggatgc?aaatcagagg?gtttgtatta 780
gtggttgaaa?acttggctaa?aaatatctgt?gaaaatctag?aacaaagtgg?tttgcccgta 840
ggtggaaatg?aaaagaaagc?caaactgtca?aatgcagtgg?ccaaaatgct?cagtaactgc 900
ccaccgggag?ggatcagcat?gacagtaaca?ggagacaata?ctaaatggaa?tgaatgctta 960
aatccaagaa?tctttttggc?tatgactgaa?agaataacca?gagacagccc?aatttggttc 1020
cgggattttt?gtagtatagc?accggtcttg?ttctccaata?aaatagccag?attgggaaaa 1080
ggatttatgg?taacaagtaa?aacaaaaaga?ctgaaggctc?aaataccttg?tcctgatctg 1140
tttagcatac?cattagaaag?atataatgaa?gaaacaaggg?caaaattaag?aaagctgaaa 1200
ccattcttca?atgaagaagg?aacggcatct?ttgtcgcctg?gaatgatgat?gggaatgttt 1260
aatatgctat?ctaccgtgtt?gggagtagcc?gcactaggta?tcaaaaacat?tggaaacaaa 1320
gaatacttat?gggatggact?gcaatcttct?gatgattttg?ctctgtttgt?taatgcaaaa 1380
gatgaagaga?catgtatgga?agggataaac?gacttttacc?gaacatgtaa?attattggga 1440
ataaatatga?gcaaaaagaa?aagttactgt?aacgaaactg?gaatgtttga?atttacaagc 1500
atgttctata?gagatggatt?tgtatctaat?tttgcaatgg?aaattccttc?atttggagtt 1560
gctggagtaa?atgaatcagc?agatatggca?ataggaatga?caataataaa?gaacaatatg 1620
attaacaatg?ggatgggccc?agcaacagca?caaacagcca?tacaattgtt?catagctgat 1680
tataggtaca?cctacaaatg?ccacagggga?gattccaaag?tggaaggaaa?aagaatgaaa 1740
attataaagg?agctatggga?aaacactaaa?ggaagagatg?gtctgttagt?ggcagatggt 1800
gggcccaaca?tttacaattt?gagaaactta?catatcccag?aaatagtgtt?gaagtacaat 1860
ctaatggacc?ctgaatacaa?agggcggtta?cttcatcctc?aaaatccctt?tgtaggacat 1920
ttgtctattg?aaggcatcaa?agaagcagat?ataaccccag?cacatggtcc?cgtgaagaaa 1980
atggattatg?atgcagtatc?tgggactcat?agttggagaa?ctaaaaggaa?cagatctata 2040
ctaaatactg?atcagaggaa?catgattctt?gaggaacaat?gctacgctaa?gtgttgcaac 2100
ctttttgagg?cctgttttag?cagtgcatca?tacaggaaac?cagtaggtca?gcacagcatg 2160
cttgaagcta?tggcccatag?attaagaatg?gatgcacgac?tagattatga?atcaggaaga 2220
atgtcaaagg?atgattttga?gaaagcaatg?gctcaccttg?gtgagattgg?gtacacataa 2280
gctccgaaga?tgtctatggg?gttattggtc?atcattggat?acatgtgata?aacaaatgat 2340
taaaatgaaa?aaaggctcgt?gtttctact 2369
Claims (13)
1, a kind of new Influenza B virus complete genome sequence with mammalian cell high yield feature is characterized in that this sequence comprises sequence 1, sequence 2, sequence 3, sequence 4, sequence 5, sequence 6, sequence 7, sequence 8.
2, a kind of plasmid that includes the described Influenza B virus gene order of claim 1.
3, plasmid according to claim 1 is characterized in that described plasmid comprises: PCDNA3.1-BPB1, PCDNA3.1-BPB2, PCDNA3.1-BPA, PCDNA3.1-BNP, PCDNA3.1-BHA, PCDNA3.1-BNA, PCDNA3.1-BNS, PCDNA-3.1-BM, PHH21-BPB1, PHH21-BPB2, PHH21-PA, PHH21-NP, PHH21-HA, PHH21-NA, PHH21-NS, PHH21-BM, PIVVII-BNS, PIIV II-BM, PIVV II-BHA, PIVV II-BNA, PIVV II-BNP, PIVV II-BPA, PIVV II-BPB2, PIVV II-BPB1.
4, plasmid according to claim 3 is characterized in that described plasmid comprises PIVV II-BNS, PIVVII-BM, PIVV II-BHA, PIVV II-BNA, PIVV2 II-BNP, PIVV II-BPB1, PIVVII-BPB2 and PIVV-BPA.
5, one group of primer, the gene fragment of the Influenza B virus that is used to increase is characterized in that this primer comprises:
BM-NS-1:?5’-ATCGTCTCTGGGAGCAGAAGCAGAGCA-3’
BM-NS-2:?5’-GGCGTCTCGTATTAGTAGTAACAAGAG-3’
BM-U-1: 5’-AACGTCTCTGGGAGCAGAAGC-3’
BM-U-2: 5’-GGCGTCTCGTATTAGTAGAAAC-3’
BM-PA-1-:5-TTCGTCTCAGGGAGCAGAAGCGGT-3
BM-PB2-1:5-TTCGTCTCTGGGAGCAGAAGCGGAGCGTTTTTCAAG-3
BM-PB1-1:-5-TTGGTCTCAGGGAGCAGAAGCGGAGCG?TTTTAAG-3
6, a kind of recombinant virus strain that contains Influenza B virus high yield strain antigen property is characterized in that this strain contains the gene order above-mentioned just like claim 1.
7, a kind of reorganization Influenza B virus strain, it is characterized in that this strain on January 15th, 2003 in China Committee for Culture Collection of Microorganisms's common micro-organisms center preservation, B/ capital section/96/2001, its preserving number is 0880.
8, a kind of reorganization Influenza B virus strain as claimed in claim 6 is characterized in that it is adapted at growing on the mammalian cell.
9, reorganization Influenza B virus strain according to claim 8 is characterized in that described mammalian cell is mdck cell and/or human embryo kidney (HEK) epithelial cell 293T cell.
10, a kind of Influenza B virus strain is characterized in that its gene order comprises the sequence 1 in the claim 1, sequence 2, sequence 5, sequence 6, sequence 7, the HA of sequence 8 and popular Influenza B virus strain, NA sequence.
11, a kind of deactivation of Influenza B virus strain as claimed in claim 10 and/or second type influenza virus vaccine of attenuation of containing.
12, a kind of method for preparing new Influenza B virus strain, this method may further comprise the steps:
Use primer BM-NS-1, BM-NS-2, BM-U-1, BM-U-2, BM-PA-1, BM-PB1-1 and BM-PB2-1 amplify the full genomic fragment of Influenza B virus;
Genomic fragment is linked to each other with PIVV II carrier;
With the PIVV II plasmid transfection 293T and the MDCK co-cultured cell that contain described genomic fragment that obtains;
The supernatant liquor that contains influenza virus of results transfection.
13, a kind of method for preparing the second type influenza virus vaccine, this method may further comprise the steps:
On MDCK, cultivate the virus strain of reprovision; Collect this cell culture supernatant; Centrifugal removal fragment; Ultrafiltration obtains concentrating recombinant virus, and wherein said reprovision virus strain is meant and contains sequence 1 of the present invention, sequence 2, sequence 5, sequence 6, sequence 7, the HA of sequence 8 and popular influenza virus strain, NA sequence.
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Cited By (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| EP1856271A4 (en) * | 2005-03-08 | 2009-11-18 | Medimmune Vaccines Inc | Influenza hemagglutinin and neuraminidase variants |
| CN102149405A (en) * | 2008-07-11 | 2011-08-10 | 米迪缪尼股份有限公司 | Influenza hemagglutinin and neuraminidase variants |
| US8048430B2 (en) | 2003-06-16 | 2011-11-01 | Medimmune, Llc | Influenza hemagglutinin and neuraminidase variants |
| CN104278014A (en) * | 2006-08-09 | 2015-01-14 | 米迪缪尼有限公司 | Influenza hemagglutinin and neuraminidase variants |
-
2003
- 2003-04-10 CN CNB031218075A patent/CN100482788C/en not_active Expired - Fee Related
Cited By (11)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US8048430B2 (en) | 2003-06-16 | 2011-11-01 | Medimmune, Llc | Influenza hemagglutinin and neuraminidase variants |
| US8404248B2 (en) | 2003-06-16 | 2013-03-26 | Medimmune, Llc | Reassortant influenza B viruses |
| US8685410B2 (en) | 2003-06-16 | 2014-04-01 | Medimmune, Llc | Influenza hemagglutinin and neuraminidase variants |
| US8877210B2 (en) | 2003-06-16 | 2014-11-04 | Medimmune, Llc | Influenza hemagglutinin and neuraminidase variants |
| EP1856271A4 (en) * | 2005-03-08 | 2009-11-18 | Medimmune Vaccines Inc | Influenza hemagglutinin and neuraminidase variants |
| US8333975B2 (en) | 2005-03-08 | 2012-12-18 | Medimmune, Llc | Influenza hemagglutinin and neuraminidase variants |
| US8574593B2 (en) | 2005-03-08 | 2013-11-05 | Medimmune, Llc | Influenza hemagglutinin and neuraminidase variants |
| US8691239B2 (en) | 2005-03-08 | 2014-04-08 | Medimmune, Llc | Influenza hemagglutinin and neuraminidase variants |
| CN104278014A (en) * | 2006-08-09 | 2015-01-14 | 米迪缪尼有限公司 | Influenza hemagglutinin and neuraminidase variants |
| CN102149405A (en) * | 2008-07-11 | 2011-08-10 | 米迪缪尼股份有限公司 | Influenza hemagglutinin and neuraminidase variants |
| US8591914B2 (en) | 2008-07-11 | 2013-11-26 | Medimmune, Llc | Influenza hemagglutinin and neuraminidase variants |
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| CN100482788C (en) | 2009-04-29 |
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