Analysis of Bacillus subtilis 168 prophage-associated lytic enzymes; identification and characterization of CWLA-related prophage proteins.

S J Foster
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引用次数: 23

Abstract

The CWLA lytic amidase of Bacillus subtilis 168 was purified and antisera raised against the purified protein. No expression of cwlA could be demonstrated under any conditions by the use of the antisera and cwlA::lacZ fusion analysis. Two lytic enzymes of apparent molecular masses 34 and 30 kDa (as measured by renaturing SDS-PAGE) were found to be mitomycin C-inducible, the larger of which corresponds to a protein immunologically related to CWLA. Both of these inducible lysins were found to be encoded by prophage PBSX. Prophage SP beta was shown by renaturing SDS-PAGE to produce a 43 kDa lytic enzyme unrelated immunologically to CWLA. The smaller of the two PBSX enzymes was purified and found to be an N-acetylmuramyl-L-alanine amidase of 32 kDa (as measured by SDS-PAGE and Coomassie blue staining) which cross-reacts only weakly with the anti-CWLA sera. The potential origin of cwlA and its possible relationship to the other phage lytic enzymes are discussed.

枯草芽孢杆菌168噬菌体相关酶分析与cwla相关的噬菌体蛋白的鉴定和表征。
对枯草芽孢杆菌168的CWLA水解酶进行了纯化,并对纯化蛋白进行了抗血清的培养。使用抗血清和cwlA::lacZ融合分析,在任何条件下均未发现cwlA的表达。两种表观分子质量分别为34和30 kDa的裂解酶(通过SDS-PAGE还原测定)被发现是丝裂霉素c诱导的,其中较大的酶对应于一种与CWLA相关的免疫蛋白。这两种诱导溶酶均由噬菌体PBSX编码。通过SDS-PAGE还原显示,前噬菌体SP β产生与CWLA免疫无关的43 kDa裂解酶。两个PBSX酶中较小的酶被纯化,发现是一个32 kDa的n -乙酰muramyl- l-丙氨酸氨基酶(通过SDS-PAGE和考马西蓝染色测定),它与抗cwla血清只发生弱交叉反应。讨论了cwlA的可能来源及其与其他噬菌体裂解酶的可能关系。
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