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乳酸链球菌中的质粒:乳糖代谢和蛋白酶活性与质粒相关的证据。

Plasmids in Streptococcus lactis: evidence that lactose metabolism and proteinase activity are plasmid linked.

作者信息

Efstathiou J D, McKay L L

出版信息

Appl Environ Microbiol. 1976 Jul;32(1):38-44. doi: 10.1128/aem.32.1.38-44.1976.

Abstract

Populations of lactose positive (Lac+) and proteinase positive (Prt+) cells from Streptococcus lactis M18, C10, and ML3 grown at 39 degrees C gave rise to increasing proportions of Lac- Prt- clones. The deficiencies did not appear until after a number of generations at the elevated temperature, and the rate depended on the strain.Lac- Prt+ and Lac+ Prt- mutants were isolated after treatment with ethidium bromide. Plasmid deoxyribonucleic acid was isolated by cesium chloride-ethidium bromide equilibrium density gradient centrifugation from the parent cultures as well as from their Lac- Prt-, Lac- Prt+, and Lac+ Prt- mutants. Five distinct plasmid sizes of approximate molecular weights of 2,4, 8, 21, and 27 million were found in S. lactis C10, whereas the Lac- Prt- derivative lacked the 8- and 21-million-dalton plasmids, but the 8-million-dalton plasmid was present in the Lac-Att mutant. In S. lactis m18 five plasmids possessing molecular weights of about 2, 4, 10, 18 and 27 million were observed. The 10- and 18-million-dalton plasmids were not detected in the Lac- Prt- mutants, whereas the Lac- Prt+ derivative lacked only the 18-million-dalton plasmid and the Lac+ Prt- mutant lacked only the 10-million-dalton plasmid. In S. lactis ML3 five distinct plasmids, with approximate molecular weights of 2, 4, 8, 22, and 30 million, were present. The 8- and 22-million-dalton plasmids were not detected in the Lac- Prt- derivative, but the 8-million-dalton plasmid was present in the Lac- Prt+ mutant. The evidence suggests that lactose-fermenting ability and proteinase activity in these organisms are mediated through two distinct plasmids having molecular weights of 8 x 10(6) to 10 x 10(6) for proteinase activity and 18 x 10(6) to 22 x 10(6) for lactose metabolism.

摘要

在39摄氏度下培养的乳酸乳球菌M18、C10和ML3的乳糖阳性(Lac+)和蛋白酶阳性(Prt+)细胞群体产生了比例不断增加的Lac- Prt-克隆。这些缺陷直到在高温下传代若干次后才出现,且速率取决于菌株。用溴化乙锭处理后分离出了Lac- Prt+和Lac+ Prt-突变体。通过氯化铯-溴化乙锭平衡密度梯度离心法从亲代培养物及其Lac- Prt-、Lac- Prt+和Lac+ Prt-突变体中分离出质粒脱氧核糖核酸。在乳酸乳球菌C10中发现了五种不同大小的质粒,其近似分子量分别为200万、400万、800万、2100万和2700万,而Lac- Prt-衍生物缺少800万和2100万道尔顿的质粒,但800万道尔顿的质粒存在于Lac-Att突变体中。在乳酸乳球菌m18中观察到了五种分子量约为200万、400万、1000万、1800万和2700万的质粒。在Lac- Prt-突变体中未检测到1000万和1800万道尔顿的质粒,而Lac- Prt+衍生物仅缺少1800万道尔顿的质粒,Lac+ Prt-突变体仅缺少1000万道尔顿的质粒。在乳酸乳球菌ML3中存在五种不同的质粒,其近似分子量分别为200万、400万、800万、2200万和3000万。在Lac- Prt-衍生物中未检测到800万和2200万道尔顿的质粒,但800万道尔顿的质粒存在于Lac- Prt+突变体中。证据表明,这些生物体中的乳糖发酵能力和蛋白酶活性是由两种不同的质粒介导的,蛋白酶活性的质粒分子量为8×10⁶至10×10⁶,乳糖代谢的质粒分子量为18×10⁶至22×10⁶。

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