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A 20-KILODALTON PROTEIN PRESERVES CELL VIABILITY AND PROMOTES CYTA CRYSTAL-FORMATION DURING SPORULATION IN BACILLUS-THURINGIENSIS

被引:106
作者
WU, D
FEDERICI, BA
机构
[1] UNIV CALIF RIVERSIDE,DEPT ENTOMOL,RIVERSIDE,CA 92521
[2] UNIV CALIF RIVERSIDE,INTERDEPARTMENTAL GRAD PROGRAM GENET,RIVERSIDE,CA 92521
来源
JOURNAL OF BACTERIOLOGY | 1993年 / 175卷 / 16期
关键词
D O I
10.1128/JB.175.16.5276-5280.1993
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
The effect of a 20-kDa protein on cell viability and CytA crystal production in its natural host, Bacillus thuringiensis, was studied by expressing the cytA gene in the absence or presence of this protein. In the absence of the 20-kDa protein, B. thuringiensis cells either were killed during sporulation (strain cryB) or produced very small CytA crystals (strain 4Q7). Expression of cytA in the presence of the 20-kDa protein, however, preserved cell viability, especial[y in strain cryB, and in both strains yielded bipyramidal crystals of the CytA protein that were larger than those of wild-type B. thuringiensis. These results suggest that the 20-kDa protein promotes crystal formation, perhaps by chaperoning CytA molecules during synthesis and crystallization, concomitantly preventing the CytA protein from interacting lethally with the bacterial host cell.
引用
收藏
页码:5276 / 5280
页数:5
相关论文
共 27 条
[1]   A 20-KILODALTON PROTEIN IS REQUIRED FOR EFFICIENT PRODUCTION OF THE BACILLUS-THURINGIENSIS SUBSP ISRAELENSIS 27-KILODALTON CRYSTAL PROTEIN IN ESCHERICHIA-COLI [J].
ADAMS, LF ;
VISICK, JE ;
WHITELEY, HR .
JOURNAL OF BACTERIOLOGY, 1989, 171 (01) :521-530
[2]   PROPERTIES OF A 72-KILODALTON MOSQUITOCIDAL PROTEIN FROM BACILLUS-THURINGIENSIS SUBSP MORRISONI PG-14 EXPRESSED IN BACILLUS-THURINGIENSIS SUBSP KURSTAKI BY USING THE SHUTTLE VECTOR PHT3101 [J].
CHANG, C ;
DAI, SM ;
FRUTOS, R ;
FEDERICI, BA ;
GILL, SS .
APPLIED AND ENVIRONMENTAL MICROBIOLOGY, 1992, 58 (02) :507-512
[3]   INVOLVEMENT OF A POSSIBLE CHAPERONIN IN THE EFFICIENT EXPRESSION OF A CLONED CRYIIA DELTA-ENDOTOXIN GENE IN BACILLUS-THURINGIENSIS [J].
CRICKMORE, N ;
ELLAR, DJ .
MOLECULAR MICROBIOLOGY, 1992, 6 (11) :1533-1537
[4]  
CRICKMORE N, 1990, ASPECTS APPL BIOL, V24, P17
[5]   DELETION BY INVIVO RECOMBINATION SHOWS THAT THE 28-KILODALTON CYTOLYTIC POLYPEPTIDE FROM BACILLUS-THURINGIENSIS SUBSP ISRAELENSIS IS NOT ESSENTIAL FOR MOSQUITOCIDAL ACTIVITY [J].
DELECLUSE, A ;
CHARLES, JF ;
KLIER, A ;
RAPOPORT, G .
JOURNAL OF BACTERIOLOGY, 1991, 173 (11) :3374-3381
[6]   MOLECULAR CHARACTERIZATION OF A GENE ENCODING A 72-KILODALTON MOSQUITO-TOXIC CRYSTAL PROTEIN FROM BACILLUS-THURINGIENSIS SUBSP ISRAELENSIS [J].
DONOVAN, WP ;
DANKOCSIK, C ;
GILBERT, MP .
JOURNAL OF BACTERIOLOGY, 1988, 170 (10) :4732-4738
[7]   SENSITIVITY TO PLATING OF ESCHERICHIA-COLI-CELLS EXPRESSING THE CRYA GENE FROM BACILLUS-THURINGIENSIS VAR ISRAELENSIS [J].
DOUEK, J ;
EINAV, M ;
ZARITSKY, A .
MOLECULAR & GENERAL GENETICS, 1992, 232 (01) :162-165
[8]   MOLECULAR CHAPERONES [J].
ELLIS, RJ ;
VANDERVIES, SM .
ANNUAL REVIEW OF BIOCHEMISTRY, 1991, 60 :321-347
[9]   PLASMID LOCATION, CLONING, AND SEQUENCE-ANALYSIS OF THE GENE ENCODING A 27.3-KILODALTON CYTOLYTIC PROTEIN FROM BACILLUS-THURINGIENSIS SUBSP MORRISONI (PG-14) [J].
GALJART, NJ ;
SIVASUBRAMANIAN, N ;
FEDERICI, BA .
CURRENT MICROBIOLOGY, 1987, 16 (03) :171-177
[10]  
HOFTE H, 1989, MICROBIOL REV, V53, P242
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