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首页> 外文OA文献 >Activation of Shiga-like toxins by mouse and human intestinal mucus correlates with virulence of enterohemorrhagic Escherichia coli O91:H21 isolates in orally infected, streptomycin-treated mice
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Activation of Shiga-like toxins by mouse and human intestinal mucus correlates with virulence of enterohemorrhagic Escherichia coli O91:H21 isolates in orally infected, streptomycin-treated mice

机译:通过小鼠和人肠粘菌激活滋生毒素与口腔感染的肠溶性大肠杆菌o91:H21分离物的毒力相关的毒力与口服感染,链霉素处理的小鼠的毒力相关

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The enterohemorrhagic Escherichia coli (EHEC) O91:H21 isolates B2F1 and H414-36/89 are virulent in an orally infected streptomycin-treated mouse model. Previous studies demonstrated that B2F1 and H414-36/89 grow to high levels in mucus isolated from the mouse small intestine and colon and that growth in smallintestinal mucus is related to virulence. We measured the levels of Shiga-like toxins (SLTs) SLT-IIvha and SLT-IIvhb produced by B2F1 after growth in Luria-Bertani (LB) broth supplemented with mouse intestinal mucus by assaying the cytotoxicity of culture supernatants on Vero cells. Culture supernatants from B2F1 grown in mouse intestinal mucus, but not EHEC strains that produce SLT-II or SLT-IIc, were approximately 35- to 350-fold more toxic for Vero cells than supernatants from B2F1 grown in LB broth. This increased toxicity was not reflected by a concomitant increase in SLT antigen content. Furthermore, when culture supernatants from B2F1 or K-12 strains carrying plasmids encoding SLTs cloned from H414-36/89 or purified SLT-IIvhb from B2F1 were incubated with mouse intestinal mucus, the samples exhibited greater cytotoxicity than when they were incubated with N-2-hydroxyethylpiperazine-Nu27-2-ethanesulfonic acid (HEPES) buffer alone. These toxin preparations also showed increased cytotoxicity after incubation with human colonic mucus. In contrast, culture supernatants from LB-grown EHEC isolates that produced SLT-I, SLT-II, SLT-IIc, or SLT-IIe did not show increased cytotoxicity after incubation with mouse or human intestinal mucus. The A subunits of purified SLT-II and SLT-IIvhb that had been treated with mouse intestinal mucus or trypsin were cleaved to A1 fragments by the mucus, but trypsin-mediated cleavage, unlike treatment with mouse intestinal mucus, did not result in increased Vero cell cytotoxic activity. This finding implies that the increased cytotoxicity of SLT-IIvhb detected after incubation with mucus is probably not due to cleavage of the A subunit into the A1 and A2 fragments. Taken together, these results indicate that mouse or human intestinal mucus directly activates SLT-II-related toxins from B2F1 and H414-36/89 and suggest that toxin activation may explain the low 50% lethal doses of B2F1 and H414-36/89 in streptomycin-treated mice.
机译:在肠出血性大肠杆菌(EHEC)O91:H21株B2F1和H414-36 / 89是在口服感染链霉素处理的小鼠模型毒性。以前的研究表明,B2F1和H414-36 / 89生长到高的水平在来自小鼠小肠和结肠和在smallintestinal粘液生长分离粘液涉及毒力。我们测量的水平志贺样毒素(SLT)连接SLT-IIvha和SLT-IIvhb产生由B2F1在通过测定在Vero细胞培养物上清液的细胞毒性补充有小鼠肠粘液的Luria-BERTANI(LB)肉汤生长之后。从B2F1培养物上清液在小鼠肠粘液中生长,但不能EHEC菌株产生SLT-II或SLT-IIC,分别为约35-至350倍的毒性的Vero细胞比从在LB肉汤B2F1生长上清液。该增加的毒性不是由在SLT抗原含量伴随增加反射。此外,当从B2F1或K-12株携带编码来自B2F1从H414-36 / 89或纯化SLT-IIvhb克隆的SLT质粒的培养物上清液与小鼠肠粘液孵育,所述样品表现出比当它们与N-孵育更大的细胞毒性2-羟乙基-N u27-2乙磺酸(HEPES)缓冲液单独。这些毒素制剂也表现出与人类结肠粘液培养后增加毒性。与此相反,从LB生长的EHEC培养物上清液分离用小鼠或人肠粘液温育后所产生SLT-I,SLT-II,SLT-IIC,或SLT-IIe上没有显示出增加的细胞毒性。已用小鼠肠粘液或胰蛋白酶处理纯化SLT-II和SLT-IIvhb的A亚单位是由粘液裂解A1片段,但胰蛋白酶介导的裂解,用小鼠肠粘液不像治疗,没有导致增加的Vero细胞毒活性。这一发现意味着,SLT-IIvhb的增加的细胞毒性,粘液可能不是由于A亚基成A1和A2片段的裂解温育后检测。总之,这些结果表明,小鼠或人肠粘液直接激活从B2F1 SLT-II相关的毒素和H414-36 / 89,并表明毒素活化可以解释低50%致死剂量的B2F1和H414-36 / 89链霉素治疗的小鼠。

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