脆弱拟杆菌TAL2480神经氨酸酶基因nanH在大肠杆菌中的克隆与表达。
Cloning and expression of the Bacteroides fragilis TAL2480 neuraminidase gene, nanH, in Escherichia coli.
作者信息
Russo T A, Thompson J S, Godoy V G, Malamy M H
机构信息
Department of Geographic Medicine and Infectious Diseases, New England Medical Center, Boston, Massachusetts.
出版信息
J Bacteriol. 1990 May;172(5):2594-600. doi: 10.1128/jb.172.5.2594-2600.1990.
We have cloned the Bacteroides fragilis TAL2480 neuraminidase (NANase) structural gene, nanH, in Escherichia coli. This was accomplished by using the cloning shuttle vector pJST61 and a partial Sau3A library of TAL2480 chromosomal inserts created in E. coli. The library was mobilized into the NANase-deficient B. fragilis TM4000 derivative TC2. NANase-producing colonies were enriched by taking advantage of the inability of TC2, but not the wild-type of NANase+ revertant, to grow in vitro in fluid aspirated from the rat granuloma pouch. Plasmids pJST61-TCN1 and pJST61-TCN3, containing inserts of 9.1 and 4.5 kilobases (kb), respectively, were found in the TC2 derivatives that grew in the rat pouch medium. In B. fragilis, NANase production from the two plasmids was inducible by free N-acetylneuraminic acid or sialic acid-containing substrates, just as in the parental TAL2480 strain. However, when these plasmids were transferred back to E. coli, NANase activity was barely detectable. A 3.5-kb portion of the insert in pJST61-TCN3 was subcloned in pJST61 to give plasmid pJST61-SC3C; NANase was produced from this plasmid both in E. coli and in B. fragilis. In E. coli, NANase expression was under the control of the vector promoter lambda pR and was therefore completely abolished by the presence of a lambda prophage. In B. fragilis, NANase production was inducible by free N-acetylneuraminic acid or sialic acid-containing substrates. By using deletion analysis and Tn1000 mutagenesis, the NANase structural gene and control region that functions in B. fragilis were localized to a 1.5- to 2.0-kb region of the insert. A partial nucleotide sequence of the NANase-deficient Tn1000 insertion mutants allowed us to identify the nanH gene and deduce the amino acid sequence of a portion of the NANase protein. We identified five regions showing great similarity to the Asp boxes, -Ser-X-Asp-X-Gly-X-Thr-Trp-, of other bacterial and viral NANase proteins.
我们已在大肠杆菌中克隆了脆弱拟杆菌TAL2480神经氨酸酶(NANase)的结构基因nanH。这是通过使用克隆穿梭载体pJST61和在大肠杆菌中构建的TAL2480染色体插入片段的部分Sau3A文库来实现的。该文库被转入NANase缺陷型脆弱拟杆菌TM4000衍生物TC2中。利用TC2(而非野生型NANase +回复株)无法在从大鼠肉芽肿袋吸出的液体中体外生长这一特性,富集产生NANase的菌落。在大鼠袋培养基中生长的TC2衍生物中发现了分别含有9.1和4.5千碱基(kb)插入片段的质粒pJST61 - TCN1和pJST61 - TCN3。在脆弱拟杆菌中,这两种质粒产生NANase可被游离的N - 乙酰神经氨酸或含唾液酸的底物诱导,就如同在亲本TAL2480菌株中一样。然而,当这些质粒被转回大肠杆菌时,几乎检测不到NANase活性。pJST61 - TCN3中插入片段的一个3.5 - kb部分被亚克隆到pJST61中,得到质粒pJST61 - SC3C;该质粒在大肠杆菌和脆弱拟杆菌中均产生NANase。在大肠杆菌中,NANase的表达受载体启动子λpR的控制,因此λ原噬菌体的存在会使其完全消失。在脆弱拟杆菌中,NANase的产生可被游离的N - 乙酰神经氨酸或含唾液酸的底物诱导。通过缺失分析和Tn1000诱变,在脆弱拟杆菌中起作用的NANase结构基因和控制区域被定位到插入片段的1.5至2.0 kb区域。NANase缺陷型Tn1000插入突变体的部分核苷酸序列使我们能够鉴定nanH基因并推导NANase蛋白一部分的氨基酸序列。我们鉴定出五个区域,它们与其他细菌和病毒NANase蛋白的Asp框(-Ser-X-Asp-X-Gly-X-Thr-Trp-)具有高度相似性。
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