AEROMONAS SPP CAN SECRETE ESCHERICHIA-COLI ALKALINE-PHOSPHATASE INTO THE CULTURE SUPERNATANT, AND ITS RELEASE REQUIRES A FUNCTIONAL GENERAL SECRETION PATHWAY

被引：11

作者：

WONG, KR ^{[1
]}

BUCKLEY, JT ^{[1
]}

机构：

[1] UNIV VICTORIA, DEPT BIOCHEM & MICROBIOL, BOX 3055, VICTORIA V8W 3P6, BC, CANADA

来源：

MOLECULAR MICROBIOLOGY | 1993年 / 9卷 / 05期

关键词：

D O I：

10.1111/j.1365-2958.1993.tb01225.x

中图分类号：

Q5 [生物化学]; Q7 [分子生物学];

学科分类号：

071010 ; 081704 ;

摘要：

Aerolysin is a channel-forming protein secreted by Aeromonas hydrophila. To determine if regions of aerolysin could direct the secretion of another protein, portions of aerA were fused to phoA, the Escherichia coli alkaline phosphatase gene and cloned into E. coli, Aeromonas salmonicida, and A. hydrophila. We were surprised to find that secretion of the enzyme by both Aeromonas spp. was independent of the aerolysin segments fused to it. The smallest fusion product contained only the signal sequence and two amino acids of aerolysin. The largest had more than 90% of the aerolysin molecule. The fusion proteins were found in the periplasms of E. coli and A. salmonicida grown in LB medium containing glucose, as well as in the shocked cells. Aerolysin itself was secreted by A. salmonicida under these conditions. In contrast, when A. salmonicida containing any of the fused genes was grown in LB medium without glucose, most of the alkaline phosphatase activity was extracellular, whereas beta-lactamase remained in its normal periplasmic location. Similar results were obtained with A. hydrophila. The change in location of the enzyme in A. salmonicida appeared to be related to the pH of the growth medium. A. salmonicida and A. hydrophila also secreted native E. coli alkaline phosphatase, but A. hydrophila strains with mutations in the general secretion pathway were unable to release the enzyme. We conclude that the Aeromonas secretion system can recognize the E. coli enzyme as an extracellular protein and direct it outside the cell.

引用

页码：955 / 963

页数：9

共 39 条

[1] CITRATE TRANSPORT IN SALMONELLA-TYPHIMURIUM - STUDIES WITH 2-FLUORO-L-ERYTHRO-CITRATE AS A SUBSTRATE [J].

ASHTON, DM ;

SWEET, GD ;

SOMERS, JM ;

KAY, WW .

CANADIAN JOURNAL OF BIOCHEMISTRY, 1980, 58 (10) :797-803

[2]

BIRNBOIM HC, 1979, BIOCHIM BIOPHYS ACTA, V299, P516

[3] ANALYSIS OF REGULATION OF ESCHERICHIA-COLI ALKALINE-PHOSPHATASE SYNTHESIS USING DELETIONS AND PHI-80 TRANSDUCING PHAGES [J].

BRICKMAN, E ;

BECKWITH, J .

JOURNAL OF MOLECULAR BIOLOGY, 1975, 96 (02) :307-316

[4] PURIFICATION OF CLONED PROAEROLYSIN RELEASED BY A LOW PROTEASE MUTANT OF AEROMONAS-SALMONICIDA [J].

BUCKLEY, JT .

BIOCHEMISTRY AND CELL BIOLOGY, 1990, 68 (01) :221-224

[5] RELEASE OF ALKALINE PHOSPHATASE FROM CELLS OF PSEUDOMONAS-AERUGINOSA BY MANIPULATION OF CATION CONCENTRATION AND OF PH [J].

CHENG, KJ ;

INGRAM, JM ;

COSTERTO.JW .

JOURNAL OF BACTERIOLOGY, 1970, 104 (02) :748-+

[6] STRUCTURE AND MECHANISM OF ALKALINE-PHOSPHATASE [J].

COLEMAN, JE .

ANNUAL REVIEW OF BIOPHYSICS AND BIOMOLECULAR STRUCTURE, 1992, 21 :441-483

[7] THE CYTOLYTIC TOXIN AEROLYSIN MUST AGGREGATE TO DISRUPT ERYTHROCYTES, AND AGGREGATION IS STIMULATED BY HUMAN GLYCOPHORIN [J].

GARLAND, WJ ;

BUCKLEY, JT .

INFECTION AND IMMUNITY, 1988, 56 (05) :1249-1253

[8] PROBING FHUA'-'PHOA FUSION PROTEINS FOR THE STUDY OF FHUA EXPORT INTO THE CELL-ENVELOPE OF ESCHERICHIA-COLI-K12 [J].

GUNTER, K ;

BRAUN, V .

MOLECULAR & GENERAL GENETICS, 1988, 215 (01) :69-75

[9] HIGH-FREQUENCY MOBILIZATION OF THE CHROMOSOME OF ESCHERICHIA-COLI BY A MUTANT OF PLASMID RP4 TEMPERATURE-SENSITIVE FOR MAINTENANCE [J].

HARAYAMA, S ;

TSUDA, M ;

IINO, T .

MOLECULAR & GENERAL GENETICS, 1980, 180 (01) :47-56

[10] CONFORMATION OF PROTEIN SECRETED ACROSS BACTERIAL OUTER MEMBRANES - A STUDY OF ENTEROTOXIN TRANSLOCATION FROM VIBRIO-CHOLERAE [J].

HIRST, TR ;

HOLMGREN, J .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1987, 84 (21) :7418-7422

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