PRODUCTION AND RELEASE OF POLYPHOSPHATE BY A GENETICALLY-ENGINEERED STRAIN OF ESCHERICHIA-COLI

被引：10

作者：

HARDOYO

YAMADA, K

SHINJO, H

KATO, J

OHTAKE, H

机构：

[1] HIROSHIMA UNIV,DEPT FERMENTAT TECHNOL,HIROSHIMA 724,JAPAN

[2] EBARA RES CO LTD,ENVIRONM PROTECT RES INST,FUJISAWA 251,KANAGAWA,JAPAN

来源：

APPLIED AND ENVIRONMENTAL MICROBIOLOGY | 1994年 / 60卷 / 10期

关键词：

D O I：

10.1128/AEM.60.10.3485-3490.1994

中图分类号：

Q81 [生物工程学（生物技术）]; Q93 [微生物学];

学科分类号：

071005 ; 0836 ; 090102 ; 100705 ;

摘要：

A recombinant strain of Escherichia coli MV1184, which contains plasmid-borne genes encoding the phosphate-specific transport (Pst) system and polyphosphate (polyP) kinase, accumulated high levels of P-i, and released polyP into the medium. PolyP could be separated from the culture supernatant by DEAE-Toyopearl 650M chromatography and identified by high-resolution P-31 nuclear magnetic resonance spectroscopy. Once E. coli recombinants accumulated high levels of polyP, they released polyP concomitantly with P-i uptake. PolyP release did not accompany the decrease in the cell density, indicating that it is not simply a result of cell lysis. PolyP release ceased when P-i became depleted in the medium and resumed upon addition of P-i to the medium. When P-i uptake was inhibited by 0.1 mM carbonyl cyanide m-chlorophenylhydrazone (CCCP), no polyP release was observed. Furthermore, neither P-i uptake nor polyp release occurred when cells were incubated at 4 degrees C. These findings suggest that the occurrence of polyP release is a possible mechanism that limits a further increase in the cellular polyP concentration in E. coli recombinants. High-resolution P-31 nuclear magnetic resonance spectroscopy also detected a surface pool of polyp in intact cells of the E. coli recombinant. The polyp resonance increased when cells were treated with EDTA and broadened upon the addition of a shift reagent, praseodymium. Although the mechanism of surface polyP accumulation is unclear, surface polyP seems to serve as the source for polyP release.

引用

下载

页码：3485 / 3490

页数：6

共 50 条

[31] SURVIVAL OF GENETICALLY ENGINEERED ESCHERICHIA-COLI IN NATURAL SOIL AND RIVER WATER
CHAO, WL
FENG, RL
JOURNAL OF APPLIED BACTERIOLOGY, 1990, 68 (04): : 319 - 325
[32] HIGH EXPRESSION OF THE PENICILLIN ACYLASE GENE IN GENETICALLY ENGINEERED ESCHERICHIA-COLI
PANBANGRED, W
UDOMBUNDITKUL, M
MEEVOOTISOM, V
ANNALS OF THE NEW YORK ACADEMY OF SCIENCES, 1990, 613 : 455 - 459
[33] Deoxycytidine production by a metabolically engineered Escherichia coli strain
Kim, Jin-Sook
Koo, Bong-Seong
Hyun, Hyung-Hwan
Lee, Hyeon-Cheol
MICROBIAL CELL FACTORIES, 2015, 14
[34] Deoxycytidine production by a metabolically engineered Escherichia coli strain
Jin-Sook Kim
Bong-Seong Koo
Hyung-Hwan Hyun
Hyeon-Cheol Lee
Microbial Cell Factories, 14
[35] PRODUCTION OF A BACTERIOLYSIN BY A HEMOLYTIC ESCHERICHIA-COLI STRAIN
JORGENSEN, SE
MUSSEN, HK
MULCAHY, PF
WU, GK
INFECTION AND IMMUNITY, 1983, 41 (03) : 1284 - 1290
[36] Hydrogen production from glycerol using a genetically engineered Escherichia coli HW2 strain
Liu, Qing
Xiong, De-Wang
Hu, Hong-Bo
Zhang, Xue-Hong
Gao Xiao Hua Xue Gong Cheng Xue Bao/Journal of Chemical Engineering of Chinese Universities, 2015, 29 (05): : 1133 - 1137
[37] IMPROVED PENICILLIN AMIDASE PRODUCTION USING A GENETICALLY ENGINEERED MUTANT OF ESCHERICHIA-COLI ATCC-11105
ROBAS, N
ZOUHEIRY, H
BRANLANT, G
BRANLANT, C
BIOTECHNOLOGY AND BIOENGINEERING, 1993, 41 (01) : 14 - 24
[38] MANIPULATION TECHNIQUES FOR THE PRODUCTION OF GENETICALLY-ENGINEERED REGULATORY ORGANISMS
SIMON, GC
ABSTRACTS OF PAPERS OF THE AMERICAN CHEMICAL SOCIETY, 1990, 200 : 181 - BIOT
[39] GENETICALLY ALTERING ESCHERICHIA-COLI
IOVINE, J
SCIENTIFIC AMERICAN, 1994, 270 (06) : 108 - 111
[40] BIOLOGICAL SAFETY ANALYSIS OF THE PRODUCTION OF HUMAN INSULIN BY GENETICALLY-ENGINEERED ESCHERICHIA-COLI K-12 CELLS .3. PLASMID TRANSFER BY NATURAL TRANSFORMATION AND TRANSDUCTION
MIESCHENDAHL, M
SCHAFFRATH, S
LENKEIT, C
DANNEBERG, G
ZENTRALBLATT FUR HYGIENE UND UMWELTMEDIZIN, 1993, 194 (03): : 262 - 270

← 1 2 3 4 5 →