首页> 美国卫生研究院文献>Epidemiology and Infection >Utilization of d-tartaric acid by Salmonella paratyphi B and Salmonella java: comparison of anaerobic plate test lead acetate test and turbidity test.
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Utilization of d-tartaric acid by Salmonella paratyphi B and Salmonella java: comparison of anaerobic plate test lead acetate test and turbidity test.

机译:副伤寒沙门氏菌B和沙门氏菌java对d-酒石酸的利用:厌氧平板试验醋酸铅试验和浊度试验的比较。

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摘要

d-Tartrate dehydrase of Salmonella java is an oxygen-sensitive enzyme active in cultures incubated under the poorly aerated conditions of static culture but not in fully aerated shaken cultures nor on plates incubated aerobically. On plates of d-tartrate minimal agar incubated anaerobically the enzyme or the degradation products of d-tartrate are exported from d-tartrate-positive cells and are available to d-tartrate-negative bacteria. This may give misleading growth results when d-tartrate-positive and d-tartrate-negative strains are tested for growth on the same plate of d-tartrate minimal agar. The lead-acetate test terminated at 24 h, the 24 h turbidity test and the ability to grow on d-tartrate minimal agar within 48 h differentiated 53 S. paratyphi B strains that were negative in each of the three tests from 76 S. java that were positive in each of the tests. An intermediate group of eight strains utilized d-tartrate in Difco bacto-peptone water to give a positive lead acetate reaction at 2 days, were stimulated to a varying degree by d-tartrate in Oxoid peptone water within the same period of incubation and grew poorly on d-tartrate minimal agar. These latter strains may be deficient in a permease controlling uptake of d-tartrate or export of d-tartrate dehydrase. Inability to utilize d-tartrate is unlikely to be the single character accountable for the reputed enhanced pathogenicity of S. paratyphi B when compared with S. java. Indications for the existence of an enzyme, complementary to and mutually exclusive with d-tartrate dehydrase, that has a positive correlation with pathogenicity are discussed.
机译:沙门氏菌java的d-酒石酸脱水酶是一种对氧敏感的酶,在静态曝气条件较差的条件下培养的培养物中有活性,但在完全曝气的摇动培养物中或需氧培养的培养皿中均不起作用。在无酒培养的酒石酸d-酒石酸盐平板上,酶或酒石酸d的降解产物从酒石酸d阳性细胞中输出,可用于酒石酸阴性的细菌。当在同一d-酒石酸最小琼脂平板上测试d-酒石酸阳性和d-酒石酸阴性菌株的生长时,这可能会给出令人误解的生长结果。乙酸铅测试在24小时结束,24小时浊度测试和在48小时内在d-酒石酸最小琼脂上生长的能力将53副伤寒沙门氏菌B菌株与76 S. java的三项测试中的每项均阴性在每个测试中都是阳性的。八种菌株的中间组在Difco细菌蛋白Di水中利用d-酒石酸在2天时产生乙酸铅阳性反应,在相同的孵育时间内被d-酒石酸在Oxoid蛋白ept水中刺激到不同程度,并且生长不良在d-酒石酸最小琼脂上。后面这些菌株可能缺乏控制D-酒石酸摄取或D-酒石酸脱水酶输出的通透酶。与爪哇沙门氏菌相比,不能利用d-酒石酸可能是造成副伤寒沙门氏菌B致病性增强的唯一原因。讨论了与d-酒石酸脱水酶互补并相互排斥的酶的存在指示,该酶与致病性呈正相关。

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