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Characterization of the pneumococcal bacteriophage HB-3 amidase: cloning and expression in Escherichia coli.

机译:肺炎球菌噬菌体HB-3酰胺酶的特性:在大肠杆菌中的克隆和表达。

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摘要

HB-3, a temperate bacteriophage of Streptococcus pneumoniae, synthesizes its own murein hydrolase activity when multiplying on cultures of pneumococcus. The enzyme (HBL) was purified and biochemically characterized as an N-acetylmuramoyl-L-alanine amidase of 36,000 daltons, and a 2.1-kilobase DraI fragment containing the lysin gene (hbl) was cloned and expressed in Escherichia coli. Our results demonstrated that the primary product of the hbl gene is a form with low enzyme activity that can be converted to a more active form under conditions similar to those previously described for the major pneumococcal autolysin (E. García, J.L. García, C. Ronda, P. García, and R. López, Mol. Gen. Genet. 201:225-230, 1985). The phage-encoded amidase requires the presence of choline in the teichoic acids of the pneumococcal cell walls for in vivo and in vitro activity. Comparative biochemical and immunological tests of the phage-encoded and host amidases revealed a remarkable similarity between these enzymes, although analyses of their N-terminal amino acid sequences allowed us to conclude that the amidases are similar but not identical. This appears to be the first description of the cloning of a phage-encoded amidase in gram-positive bacteria.
机译:HB-3是一种肺炎链球菌的温带噬菌体,当在肺炎球菌培养物中繁殖时,会合成其自身的murein水解酶活性。纯化该酶(HBL),并将其生化鉴定为36,000道尔顿的N-乙酰基muramoyl-L-丙氨酸酰胺酶,并克隆一个含有溶素基因(hbl)的2.1碱基碱基的DraI片段,并在大肠杆菌中表达。我们的结果表明,hbl基因的主要产物是一种酶活性低的形式,可以在类似于先前针对主要肺炎球菌自溶素(E.García,JLGarcía,C。Ronda ,P。García和R.López,分子遗传学,遗传学201:225-230,1985)。为了体内和体外活性,噬菌体编码的酰胺酶需要在肺炎球菌细胞壁的壁酸中存在胆碱。噬菌体编码和宿主酰胺酶的比较生化和免疫学测试显示,这些酶之间存在着显着的相似性,尽管对其N末端氨基酸序列的分析使我们得出结论,酰胺酶是相似但不相同的。这似乎是克隆革兰氏阳性细菌中噬菌体编码的酰胺酶的第一个描述。

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