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来自大肠杆菌的溶血素(HlyA)的活性形式和非活性形式。

Active and inactive forms of hemolysin (HlyA) from Escherichia coli.

作者信息

Wagner W, Kuhn M, Goebel W

机构信息

Institut für Genetik und Mikrobiologie, Universität Würzburg.

出版信息

Biol Chem Hoppe Seyler. 1988 Jan;369(1):39-46. doi: 10.1515/bchm3.1988.369.1.39.

Abstract

The HlyA protein (Mr 110 kDa) which is the gene product of the hlyA gene encoded by the hemolysin determinant of Escherichia coli (Goebel, W. & Hedgpeth, J. (1982) J. Bacteriol. 151, 1290-1298) was observed to accumulate in the culture supernatant (in the presence of the three other Hly proteins HlyC, B and D) throughout the active growth cycle. However, the amount of extracellular HlyA protein did not correlate with the external hemolytic activity, which declined when the cells entered the stationary phase. External hemolytic activity was highly sensitive to phospholipase C and to ultrasonication. The size of the HlyA protein on SDS-PAGE was not changed by these treatments although the hemolytic activity was entirely abolished. On a polyacrylamide gel containing 2M urea but only 0.1% SDS hemolytically active HlyA migrated slightly ahead of the inactive HlyA suggesting that HlyA is more negatively charged than HlyA. Active hemolysin from unconcentrated hemolytic supernatants migrated on Sephacryl S-400 and on glycerol gradients as large complexes. Analysis of the hemolytically active fractions on SDS-PAGE yielded in both cases only HlyA (110 kDA) as major protein. An internal hemolytic activity appeared in most Escherichia coli K-12 strains in the stationary phase which was independent of the presence of HlyA or any other Hly gene product. This hemolytic activity which reached in some strains about 10% of the level determined by the hly genes was sensitive to proteinase K and disappeared upon shift of the cells to the logarithmic phase.

摘要

HlyA蛋白(分子量110 kDa)是大肠杆菌溶血素决定簇编码的hlyA基因的产物(Goebel, W. & Hedgpeth, J. (1982) J. Bacteriol. 151, 1290 - 1298),在整个活跃生长周期中(在其他三种Hly蛋白HlyC、B和D存在的情况下),可观察到它在培养上清液中积累。然而,细胞外HlyA蛋白的量与外部溶血活性并不相关,当细胞进入稳定期时,外部溶血活性下降。外部溶血活性对磷脂酶C和超声处理高度敏感。尽管溶血活性完全丧失,但这些处理并未改变SDS - PAGE上HlyA蛋白的大小。在含有2M尿素但仅0.1% SDS的聚丙烯酰胺凝胶上,具有溶血活性的HlyA迁移速度略快于无活性的HlyA,这表明HlyA比HlyA带更多负电荷。未浓缩溶血上清液中的活性溶血素在Sephacryl S - 400和甘油梯度上以大复合物形式迁移。对SDS - PAGE上具有溶血活性的组分进行分析,在两种情况下均仅得到HlyA(110 kDA)作为主要蛋白质。在大多数大肠杆菌K - 12菌株的稳定期出现了一种内部溶血活性,它与HlyA或任何其他Hly基因产物的存在无关。这种溶血活性在某些菌株中达到由hly基因测定水平的约10%,对蛋白酶K敏感,并且在细胞转移至对数期时消失。

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