前苏联专利SU1443806A3 Method of constructing plasmodium vector phc314 or phc312 or phc624

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专利摘要:
Plasmid vectors and a process for the preparation thereof are disclosed having the same replication region as pBR322, but which have a substantially higher copy number per cell. The plasmid vectors contain a G->T point mutation at base pair 3074 of the pBR322 sequence which holds back synthesis of the repressor of plasmid replication, and also contain either no tetracycline resistance gene or the tetracycline resistance gene in an inactivated or weakened state.
公开号:SU1443806A3
申请号:SU843792252
申请日:1984-09-14
公开日:1988-12-07
发明作者:Борош Имре；Венетианер Пал；Пошфаи Дьердь
申请人:Рихтер Гедеон Ведьесети Дьяр Рт (Инопредприятие)；
IPC主号:

专利说明:

CN
15
20
25
114A3806
The invention relates to biotechnology, genetic engineering, and more specifically to a method for producing plasmid vectors.
The purpose of the invention is to construct plasmid vectors based on pBR322, which have a large number of copies per cell rather than known and widely used vectors, Q
Plasmid vectors pNC314, pNS312 and rNSb24 have a large number of copies due to the fact that a gene is mutated in the gene responsible for the production of plasmid replication repressor.
Example. Plasmid phC1 is cleaved with restriction endonucci ™ by EcoR1 and Pru 11 leases, and then the single ends are supplemented with the Klenow subunit JJ polymerase I in the presence of dTP substrates. The blunt ends of the DNA molecules thus obtained are reduced to the ring structure of the DNA gas. TA and transform, in HB101 cells. From the colonies growing on the medium containing ampicillin, plasmid DNA and DNA samples were obtained, which were analyzed using an agarose and polyacrylamide gel electrophoresis after digestion with restriction endonucleases EsoC1, PVU 1.1 and BspPI. Based on the total molecular weight of the plasmid (2.3 kb) and the size of the fragments obtained by the cleavage of BspP1 (587; 457, - 434j 267; 240j 80 bp), the plasmid rHC81 contains the region between nucleotides 2069 and 2 of the plasmid Q pBY22 s mutation responsible for the high number of copies.
A 1030 bp DNA fragment obtained by digestion is obtained. The pHC81 restriction endonucleases Pst1 and Tag 1, a DNA fragment of 780 bp, obtained by digestion of pBR322 with the enzymes Pst and C 1-1, and a DNA fragment of 218 bp. obtained by digestion of pBR329 with the Tag enzyme. one . Three DNA fragments obtained are mixed in equiolar ratio, stitched with DNA ligase, and HB101 cells are transformed with ligate. Plasmid DNA was isolated from individual elephants grown on ampicillin-containing medium. These plasmids have the phenotype of a large number of copies. Ras-: splinter plasmid DNA restriction 30
35
50
55
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five
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five
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Q

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By endonucleases, it is determined that they were obtained by binding three well different fragments of different origin. In these plasmids, the proximal part. The s-lactamase gene was obtained from pBR322, the site responsible for replication from the plasmid pBR322, and the fragment isolated from pHCBI contained, in addition to the distal part, the lactamase gene, also resulting in a high number of copies. Therefore, a mutation is formed between the 2573 (tagi) and 3612 (Pst1) nucleotides of the plasmid pBR322 DNA. The nucleotide sequence of this region is determined and compared to the known pBR322 sequence. As a result of this comparison, a substitution is established at position 4074 of the gene.
As a result of the resulting point mutation, the end of transcription of repressor RNA is disrupted and RNA is synthesized with a higher molecular weight, which can no longer function as a replication replication. The end of the repressor function leads to a large number of copies. Due to this spontaneous point mutation, the number of copies of the plasmid in the cell can be increased by 20-30 times (approximately 1000) with respect to the initial value. Due to this point mutation, the number of copies of any plasmid with the same replication region as pBR322 can be significantly increased.
E. coli HB101 cells are transformed with a plasmid. Plasmid DNA was isolated and analyzed by gel electrophoresis after cleavage with EcoRI and Psti with restriction endonucleases. For further studies, the plasmid is selected, which can be split into fragments 2300 and 110 bp using EcoRl and into fragments 1580 and 820 bp using Psti (pNC314). The plasmid was digested with the Baralll restriction endonuclease, and the resulting linear molecule was partially digested with the enzyme Hinf1, DNA fragments of size 2010. They were digested on a 1.2% agarose gel.
The ends of molecules containing the same sites, obtained by splitting with the enzymes BamHl and Hinfl, are converted into blunt ends of subfragmen31443806
Kleiov's volume using DNA polymerase 1, and then recirculating T-induced polynucleotide ligase. The doped DNA was transformed into IV 101 cells and isolated single colonies. The plasmid pNS312 is obtained, which cannot be cleaved with the endonuclease VatH1, but it is possible to linearize the activity in real plasmid DNA and in chromosomal DNA. In this way, the copy number of plasmids of the same size with phC314 (MB 1.6 to 10 d) was about 1000 per cell (mol. Weight of chromosome 2-10 e). From 60 to 65% of the total DP1K content of the cell is plasma DNA.
to erase EcoRI and obtain fragments of D for labeling the DNA in vivo of the cell,
1495 bp and b1 bp after cleavage of Hinf1. To obtain a vector with a large number of copies suitable for cloning DNA fragments with blunt ends, plasmid pNC312 was cleaved with restriction endonucleases EcoR1 and Ilinfll1, and then a fragment of 1980 bp was isolated from an agarose gel. This fragment is mixed with plasmid IIAN7 DNA digested with the enzymes 20 EcoRI and Hinf111, and is bound by a polynucleotide ligase. E. coli HB101 cells are transformed with a doped plasmid and from single bacterial colonies resistant to Amp, isolated plasmid DNA. The plasmid DNA obtained in this way (PHC624) does not have a C1-1 site, but, unlike the plasmid phCNS12, it can be cut with Smal, Sail, and BatH1 restriction endonucleases.
Example 2. To determine the relative copy number of the plasmid of the plasmid, E. coli HB101 cultures are grown containing plasmids of various sizes, obtained from recombinant pBR322 and derivatives with a large number of copies of the same size to achieve identical cell density. Of
containing plasmids are cultured on M9 culture medium supplemented with the following components: 0.5% casamic acid (Difco); 0.5%
15 GLUCOSES} 1 µg / ml of vitamin B; 2 mmol MgS04, 2 μg / ml thymidine 250 μg / ml adenosine and 0.4 MBg / ml (H-thymidine) 888 Bg / mole (Hemapol Prague).
Cells containing plasmids are digested. Chromosomal and plasmid DNAs are separated from each other by gradient centrifugation with ethidium bromine (cesium) chloride in equilibrium
25 density of cell lysate obtained from the bacterial suspension grown by 2 ml / OD 5 o 4-5 (45000 rpm, 40 h,).
Plasmid vectors rNS312, rNS3
30 and rNSb24 07.03.84 were deposited in the National Collection of Micro Organisms (OKI, Vengri) under the codes No. 00279, 00280 and 00281, respectively.

权利要求:
Claims (1)
[1]
Invention Formula
A method for constructing a plasmid vector pHC314 or pHC312,
identical amounts of the obtained sus-jo or pHC624, which means that
Pensions without amplification isolated plasma DNA. Samples taken from DNA preparations were subjected to electrophoretic treatment on an agarose gel in 5, 10, 15, 20, 25, 30, 40, and 50-fold dilutions, respectively. Plasmids with a large number of copies and their pairs with a normal number of copies (of the same molecular weight) are examined simultaneously. The pHCBI reagent, which contains the G T point mutation at the position 3074 of the region of the gene encoding the repressor DNA, then plasmid pH081 DNA is treated with the EcoRI endonuclease, gg is dephosphorylated by alkaline phosphatase and stitched with an EcoRI fragment of the plasmid nVX obtained by recombinant recombinant DNA obtained by recombinant DNA and synthesized with plasmid pH081; E. coli HB101 strains, amp colonies are selected, of which
Experimental results show that the number of copies of the plasmid's pNC is 20–30 times greater than the number of the corresponding pHBR322 derivatives with a normal number of copies.
Example 3. The absolute number of copies of the plasmid rHC was determined by labeling the DNA of cells containing plasmids in vivo and measuring the ratio
containing plasmids are cultured on M9 culture medium supplemented with the following components: 0.5% casamic acid (Difco); 0.5%
GLUCOSE} 1 µg / ml of vitamin B; 2 mmol MgS04, 2 μg / ml thymidine 250 μg / ml adenosine and 0.4 MBg / ml (H-thymidine) 888 Bg / mole (Hemapol, Prague).
Cells containing plasmids are cleaved. Chromosomal and plasmid DNAs are separated from each other by gradient centrifugation with ethidium bromine (cesium) chloride in equilibrium
the density of the cell lysate obtained from the bacterial suspension, grown by 2 ml / OD 5 about 4-5 (45000 rpm, 40 h,).
Plasmid vectors rNS312, rNS314
and rNSb24 07.03.84 were deposited in the National Collection of Microorganisms (OKI, Vengry) under the code number 00279, 00280 and 00281, respectively.
Invention Formula
A method for constructing a plasmid vector pHC314 or pC3312
The pHC1 plasmid DNA was digested with the EcoRI and PruII retreatment endonucleases, the ends were blunt with the Klenow subfragment of DNA-453 I in the presence of dNTP, the ring structure of the DNA was reconstructed with the DNA ligase T, and the Escherichia coli HB101 strain was transformed plasmid DNA was isolated from amp clones, digested with E. coRI and PstI endonucleases and selected for pHC314, which can be broken down into fragments of 2300 and 100 kb in size to PstI fragments of size 1580 and 820 kb, then recombinant PCA DNA PCH in the case of the construction of pNC312 cleaved with Wat HI endonuclease, the resulting linear DNA was partially hydrolyzed with the Hinfl endonuclease, a 2010 kb fragment was isolated, the circular DNA structure was reconstructed, the E. coli HB101 strain of this recombinant DNA was selected and the recombinant plasmid DNA of pHH312 was transformed,
restriction sites containing E.coRI and Hinfl and forming fragments of 1495 and 516 kb in size after digesting the plasmid E.CRI and Hinfl with plasmid rHC312; in the case of constructing the pHH66, digesting E.coRI and Hind111 with endonucleases and isolating the fragment with 1980 kb, mixed with the digested enzymes E.coRI and Hindlll DNA plasmids PAA, fragments sew DNA ligase TF, transform the strain of bacteria E. coli HB101, the resulting plasmid and from the agar clones selected recombinant plasmid DNA rNSb24 containing Sraal, Sail and BamHI sites.

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同族专利:

公开号 | 公开日

FI843600A0|1984-09-14|

PL152527B1|1991-01-31|

ZA847273B|1986-01-29|

ATA293584A|1987-02-15|

FR2552102B1|1987-09-18|

FR2552102A1|1985-03-22|

DK439784A|1985-03-17|

GB2148301A|1985-05-30|

IT1178510B|1987-09-09|

IL72952D0|1984-12-31|

CH667672A5|1988-10-31|

SE463266B|1990-10-29|

IT8422677D0|1984-09-14|

HU194307B|1988-01-28|

BE900570A|1985-03-13|

FI843600L|1985-03-17|

GB8423161D0|1984-10-17|

GB2148301B|1988-05-11|

US4703012A|1987-10-27|

DE3434041A1|1985-09-12|

FI79552C|1990-01-10|

CA1275631C|1990-10-30|

SE8404637D0|1984-09-14|

AU578041B2|1988-10-13|

JPS60156389A|1985-08-16|

FI79552B|1989-09-29|

NL8402846A|1985-04-16|

AU3307784A|1985-03-21|

SE8404637L|1985-03-17|

DK439784D0|1984-09-14|

AT384031B|1987-09-25|

PL249593A1|1985-07-16|

HUT35280A|1985-06-28|

IL72952A|1990-11-05|

引用文献:

公开号 | 申请日 | 公开日 | 申请人 | 专利标题

DE2759053A1|1977-12-30|1979-07-12|Uhlin|METHOD FOR MANUFACTURING GENE PRODUCTS FROM PLASMID DNA|

FI793884A|1978-12-26|1980-06-27|Cetus Corp|STABILA PLASMIDER MED STORT KOPIEANTAL|

CA1198067A|1981-02-27|1985-12-17|David H. Gelfand|Stable high copy number plasmids|

CA1209501A|1982-09-16|1986-08-12|Nikos Panayotatos|Expression vector|

GB8308236D0|1983-03-25|1983-05-05|Celltech Ltd|Dna vectors|

EP0126166B1|1983-05-11|1990-01-31|Fina Research S.A.|Cloning vectors comprising a restriction site bank and the construction thereof|DE3681398D1|1985-10-21|1991-10-17|Fujisawa Pharmaceutical Co|METHOD FOR THE PRODUCTION OF INSULINE-LIKE GROWTH FACTOR IAND PLASMIDE FOR THE PRODUCTION THEREOF.|

DE4136389C2|1991-03-18|1993-07-01|Hoechst Ag, 6230 Frankfurt, De|

US20040259252A1|2001-07-18|2004-12-23|Sanders Mitchell C.|Vector containing an enhanced p15a origin of replication|

WO2006081529A2|2005-01-28|2006-08-03|Nature Technology Corp.|Compositions and processes for improved plasmid dna production|

WO2007035323A1|2005-09-16|2007-03-29|Monsanto Technology Llc|Hybrid portable origin of replication plasmids|

WO2008136790A1|2007-05-02|2008-11-13|Merial Limited|Dna plasmids having improved expression and stability|

法律状态:

优先权:

申请号 | 申请日 | 专利标题

HU833212A|HU194307B|1983-09-16|1983-09-16|Process for producing plasmidvectors of high copy number|

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