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创伤弧菌几丁质酶的决定因素:几丁质酶探针的基因克隆与应用

Chitinase determinants of Vibrio vulnificus: gene cloning and applications of a chitinase probe.

作者信息

Wortman A T, Somerville C C, Colwell R R

出版信息

Appl Environ Microbiol. 1986 Jul;52(1):142-5. doi: 10.1128/aem.52.1.142-145.1986.

Abstract

To initiate study of the genetic control of chitinolytic activity in vibrios, the chitobiase gene was isolated by cloning chromosomal DNA prepared from Vibrio vulnificus. Chimeric plasmids were constructed from Sau3A I partial digests of chromosomal DNA by ligating 5 to 15-kilobase fragments into the BamHI site, i.e., in the Tcr gene, of pBR322 (Amr Tcr). The resulting plasmids were transformed into Escherichia coli DH1. Chitobiase activity of the insert-bearing clones was detected by using a chromogenic substrate, p-nitrophenyl-N-acetyl-beta, D-glucosaminide, and confirmed by the appearance of a fluorescent end product from the hydrolysis of 4-methylumbelliferyl-beta,D-N-N'-diacetylchitobiose. Endochitinase activity was demonstrated by liberation of water-soluble products produced by the degradation of [3H]chitin. Transformation of E. coli Y10R (lacY) with plasmids from chitinase-positive clones restored the lactose-positive phenotype, suggesting the presence of a permease associated with chitinase activity. Physical mapping of plasmids containing the chitinase determinants indicate that transcription of these genes in E. coli may be initiated at a V. vulnificus promoter.

摘要

为了启动对弧菌几丁质分解活性遗传控制的研究,通过克隆创伤弧菌制备的染色体DNA分离出了壳二糖酶基因。通过将5至15千碱基的片段连接到pBR322(Amr Tcr)的BamHI位点,即Tcr基因中,从染色体DNA的Sau3A I部分消化产物构建嵌合质粒。将所得质粒转化到大肠杆菌DH1中。通过使用显色底物对硝基苯基 - N - 乙酰 - β,D - 氨基葡萄糖苷检测含插入片段克隆的壳二糖酶活性,并通过4 - 甲基伞形酮基 - β,D - N,N'-二乙酰壳二糖水解产生的荧光终产物的出现来确认。通过[3H]几丁质降解产生的水溶性产物的释放证明了内切几丁质酶活性。用来自几丁质酶阳性克隆的质粒转化大肠杆菌Y10R(lacY)恢复了乳糖阳性表型,表明存在与几丁质酶活性相关的通透酶。对含有几丁质酶决定簇的质粒进行物理图谱分析表明,这些基因在大肠杆菌中的转录可能起始于创伤弧菌启动子。

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