学术探索
学术期刊
新闻热点
数据分析
智能评审

USE OF A DUAL-ORIGIN TEMPERATURE-CONTROLLED AMPLIFIABLE REPLICON FOR OPTIMIZATION OF HUMAN INTERLEUKIN-1-BETA SYNTHESIS IN ESCHERICHIA-COLI

被引:8
作者
MASHKO, SV [1 ]
MOCHULSKY, AV [1 ]
KOTENKO, SV [1 ]
LEBEDEVA, MI [1 ]
LAPIDUS, AL [1 ]
MOCHULSKAYA, NA [1 ]
IZOTOVA, LS [1 ]
VEIKO, VP [1 ]
VINETSKY, YP [1 ]
KETLINSKY, SA [1 ]
DEBABOV, VG [1 ]
机构
[1] ALL UNION HIGHLY PURE BIOL PREPARAT RES INST,LENINGRAD,USSR
来源
GENE | 1991年 / 97卷 / 02期
关键词
RECOMBINANT DNA; TGATG VECTOR; OVERLAPPON; PLASMID COPY NUMBER; PL AND PR PROMOTERS OF LAMBDA PHAGE; PROTEIN PURIFICATION;
D O I
10.1016/0378-1119(91)90060-O
中图分类号
Q3 [遗传学];
学科分类号
071007 ; 090102 ;
摘要
A new dual-replicon recombinant plasmid, pPR53-tsr, has been constructed; it is derivative of the expression vector pPR-TGATG-1 [Mashko et al., Gene 88 (1990) 121-126]. In contrast to its progenitor, pPR53-tsr is a low-copy-number (low-Cop) plasmid amplifiable in temperature-dependent fashion. In addition to both the replicon and the par locus from plasmid pSC101, providing segregational stability and a low Cop at 28-degrees-C, the new plasmid contains a mutant ColE1 replicon whose RNAII is synthesized under the control of the p(L) promoter. The presence of a thermolabile repressor, cIts857, allows the thermo-inducible amplification of pPR53-tsr; the increased plasmid Cop is estimated at approx. 200 per genome 6 h after thermal induction at 42-degrees-C. Thus, pPR53-tsr can be used as a donor of the thermo-inducible dual-replicon fragment for recombinant plasmids. Here, we employ such an approach for optimization of production of human interleukin-1-beta (hIL-1-beta) in Escherichia coli at a high level. The thermo-induced level of recombinant hIL-1-beta (re-hIL-1-beta) biosynthesis was around 9% of total cellular protein when the dual-replicon high-Cop vector was used. A method based on acidification of the water-soluble protein fraction to pH 4.0 has been developed that allows for the isolation of 80%-pure re-hIL-1-beta. The homogeneous material was obtained by two subsequent hydrophobic sorbent chromatographies. The protein yield ranged between 3-5 mg of re-hIL-1-beta/g of wet cells. The re-hIL-1-beta specific activity was about 2 X 10(8) units/mg, coinciding with that of the authentic hIL-1-beta.
引用
收藏
页码:259 / 266
页数:8
相关论文
共 36 条
[1]   COMPLETE SEQUENCE OF PSC101 [J].
BERNARDI, A ;
BERNARDI, F .
NUCLEIC ACIDS RESEARCH, 1984, 12 (24) :9415-9426
[2]   AMINO-ACID SEQUENCE-ANALYSIS OF HUMAN INTERLEUKIN-1 (IL-1) - EVIDENCE FOR BIOCHEMICALLY DISTINCT FORMS OF IL-1 [J].
CAMERON, P ;
LIMJUCO, G ;
RODKEY, J ;
BENNETT, C ;
SCHMIDT, JA .
JOURNAL OF EXPERIMENTAL MEDICINE, 1985, 162 (03) :790-801
[3]   CONSTRUCTION AND CHARACTERIZATION OF NEW CLONING VEHICLES .5. MOBILIZATION AND CODING PROPERTIES OF PBR322 AND SEVERAL DELETION DERIVATIVES INCLUDING PBR327 AND PBR328 [J].
COVARRUBIAS, L ;
CERVANTES, L ;
COVARRUBIAS, A ;
SOBERON, X ;
VICHIDO, I ;
BLANCO, A ;
KUPERSZTOCHPORTNOY, YM ;
BOLIVAR, F .
GENE, 1981, 13 (01) :25-35
[4]   MECHANISM OF CONTROL OF DNA-REPLICATION AND INCOMPATIBILITY IN COLE1-TYPE PLASMIDS - A REVIEW [J].
DAVISON, J .
GENE, 1984, 28 (01) :1-15
[5]   FUNCTIONAL DISSECTION OF ESCHERICHIA-COLI PROMOTERS - INFORMATION IN THE TRANSCRIBED REGION IS INVOLVED IN LATE STEPS OF THE OVERALL PROCESS [J].
KAMMERER, W ;
DEUSCHLE, U ;
GENTZ, R ;
BUJARD, H .
EMBO JOURNAL, 1986, 5 (11) :2995-3000
[6]   FORMATION OF RECOMBINANT PROTEIN INCLUSION-BODIES IN ESCHERICHIA-COLI [J].
KANE, JF ;
HARTLEY, DL .
TRENDS IN BIOTECHNOLOGY, 1988, 6 (05) :95-101
[7]   NEW VERSATILE CLONING AND SEQUENCING VECTORS BASED ON BACTERIOPHAGE-M13 [J].
KIENY, MP ;
LATHE, R ;
LECOCQ, JP .
GENE, 1983, 26 (01) :91-99
[8]   PURIFICATION AND CHARACTERIZATION OF RECOMBINANT HUMAN INTERLEUKIN-1-BETA PRODUCED IN ESCHERICHIA-COLI [J].
KIKUMOTO, Y ;
HONG, YM ;
NISHIDA, T ;
NAKAI, S ;
MASUI, Y ;
HIRAI, Y .
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS, 1987, 147 (01) :315-321
[9]  
KOTENKO SV, 1989, DOKL AKAD NAUK SSSR+, V309, P1005
[10]   PURIFICATION AND CHARACTERIZATION OF HUMAN INTERLEUKIN-1 EXPRESSED IN ESCHERICHIA-COLI [J].
KRONHEIM, SR ;
CANTRELL, MA ;
DEELEY, MC ;
MARCH, CJ ;
GLACKIN, PJ ;
ANDERSON, DM ;
HEMENWAY, T ;
MERRIAM, JE ;
COSMAN, D ;
HOPP, TP .
BIO-TECHNOLOGY, 1986, 4 (12) :1078-1082
1234