Braun V, Neuss B, Ruan Y, Schiebel E, Schöffler H, Jander G
J Bacteriol. 1987 May;169(5):2113-20. doi: 10.1128/jb.169.5.2113-2120.1987.
A cosmid bank of Serratia marcescens was established from which DNA fragments were cloned into the plasmid pBR322, which conferred the chromosomally encoded hemolytic activity to Escherichia coli K-12. By transposon mutagenesis with Tn1000 and Tn5 IS50L::phoA (TnphoA), the coding region was assigned to a DNA fragment, designated hly, comprising approximately 7 kilobases. Two proteins with molecular weights of 61,000 (61K protein) and 160,000 (160K protein) were expressed by the pBR322 derivatives and by a plasmid which contained the hly genes under the control of a phage T7 promoter and the T7 RNA polymerase. When strongly overexpressed the 160K protein was released by E. coli cells into the extracellular medium concomitant with hemolytic activity. The genes encoding the 61K and the 160K proteins were transcribed in the same direction. Mutants expressing a 160K protein truncated at the carboxy-terminal end were partially hemolytic. Hemolysis was progressively inhibited by saccharides with increasing molecular weights from maltotriose (Mr 504) to maltoheptaose (Mr 1,152) and was totally abolished by dextran 4 (Mr 4,000). This result and the observed influx of [14C]sucrose into erythrocytes in the presence of hemolytic E. coli transformants under osmotically protective conditions suggest the formation of defined transmembrane channels by the hemolysin.
建立了粘质沙雷氏菌的黏粒文库,从中将DNA片段克隆到质粒pBR322中,该质粒赋予大肠杆菌K-12染色体编码的溶血活性。通过用Tn1000和Tn5 IS50L::phoA(TnphoA)进行转座子诱变,将编码区域定位到一个名为hly的DNA片段上,该片段约含7千碱基。pBR322衍生物以及一个在噬菌体T7启动子和T7 RNA聚合酶控制下含有hly基因的质粒表达了两种分子量分别为61,000(61K蛋白)和160,000(160K蛋白)的蛋白质。当160K蛋白大量过表达时,大肠杆菌细胞将其释放到细胞外培养基中,同时伴有溶血活性。编码61K和160K蛋白的基因转录方向相同。表达在羧基末端截短的160K蛋白的突变体具有部分溶血活性。从麦芽三糖(Mr 504)到麦芽七糖(Mr 1,152),随着分子量增加,糖类对溶血的抑制作用逐渐增强,而葡聚糖4(Mr 4,000)则完全消除了溶血作用。这一结果以及在渗透保护条件下,溶血的大肠杆菌转化体存在时观察到的[14C]蔗糖流入红细胞的现象表明,溶血素形成了特定的跨膜通道。
