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地衣芽孢杆菌的囊泡青霉素酶:周质释放因子的存在。

Vesicle penicillinase of Bacillus licheniformis: existence of periplasmic-releasing factor(s).

作者信息

Traficante L J, Lampen J O

出版信息

J Bacteriol. 1977 Jan;129(1):184-90. doi: 10.1128/jb.129.1.184-190.1977.

Abstract

In earlier studies of the membrane-bound penicillinase of Bacillus licheniformis 749/C, the enzyme present in the vesicles that were released during protoplast formation and the enzyme retained in the plasma membrane of protoplasts appeared to differ (i) in their behavior on gel permeation chromatography in the presence or absence of deoxycholate and (ii) in their tendency to convert to the hydrophilic exoenzyme (Sargent and Lampen, 1970). We have now shown that these vesicle preparations contain a soluble, heat-sensitive enzyme(s) that is released along with the vesicles during protoplast formation. The enzyme will convert the vesicle penicillinase to a form that resembles exopenicillinase, and this conversion can be inhibited by deoxycholate under certain circumstances. Sedimentation of such vesicle preparations at 100,000 X g produces vesicles which contain penicillinase that behaves as the plasma membrane enzyme obtained from protoplasts. Exopenicillinases released by growing cells at pH 6.5 and by washed cells or protoplasts at pH 9.0 have the same NH2-terminal residues (lysine and some glutamic acid); in addition, the various release systems show a parallel sensitivity to inhibition by deoxycholate, quinacrine, chloroquine, and o-phenanthroline. The formation of exopenicillinase (by cleavage of the membrane-bound enzyme) may well be dependent on the action of the releasing enzyme.

摘要

在早期对地衣芽孢杆菌749/C膜结合青霉素酶的研究中,原生质体形成过程中释放的囊泡中存在的酶与保留在原生质体质膜中的酶似乎存在差异:(i)在有无脱氧胆酸盐存在的情况下,它们在凝胶渗透色谱上的行为不同;(ii)它们转化为亲水性外切酶的倾向不同(萨金特和兰彭,1970年)。我们现在已经表明,这些囊泡制剂含有一种可溶性的、热敏感的酶,在原生质体形成过程中与囊泡一起释放。这种酶会将囊泡青霉素酶转化为类似外切青霉素酶的形式,在某些情况下,脱氧胆酸盐可以抑制这种转化。在100,000×g的条件下对这种囊泡制剂进行沉降,会产生含有青霉素酶的囊泡,其行为与从原生质体获得的质膜酶相同。在pH 6.5时生长细胞释放的外切青霉素酶以及在pH 9.0时洗涤过的细胞或原生质体释放的外切青霉素酶具有相同的NH2末端残基(赖氨酸和一些谷氨酸);此外,各种释放系统对脱氧胆酸盐、喹吖因、氯喹和邻菲罗啉的抑制表现出相似的敏感性。外切青霉素酶的形成(通过膜结合酶的裂解)很可能依赖于释放酶的作用。

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