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Genetic Transformation of Streptococcus sanguis (Challis) with Cryptic Plasmids from Streptococcus ferus

机译:费氏链球菌隐性质粒对血链球菌的遗传转化

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By using the basic methodology initially published by Kretschmer et al. (J. Bacteriol. >124:225-231, 1975), we have been able to introduce phenotypically cryptic plasmids from Streptococcus ferus (formerly Streptococcus mutans subsp. ferus) into Streptococcus sanguis by genetic transformation. In this system, the entry of the cryptic plasmids is selected indirectly. This is effected with transforming deoxyribonucleic acid mixtures in which the cryptic plasmid deoxyribonucleic acid is present in an approximate 10-fold molar excess with respect to a plasmid (pVA1) known to confer erythromycin resistance. Under such conditions, 5 to 10% of the pVA1-containing erythromycin-resistant transformants were cotransformed with cryptic plasmid deoxyribonucleic acid. pVA1 may be selectively eliminated by growth of its S. sanguis host strain at 42°C, enabling the construction of isogenic strains with and without S. ferus cryptic plasmids. Comparative physiological studies of such strains have failed to reveal any plasmid-conferred phenotypes in S. sanguis. With this procedure, we have been able to physically separate two small cryptic plasmids (2.4 × 106 and 2.8 × 106 daltons) of S. ferus. Although these plasmids were found naturally to exist in a single S. ferus host, they were able to replicate independently of one another in S. sanguis. Restriction enzyme fingerprinting indicated that these plasmids did not share a common ancestry.
机译:通过使用最初由Kretschmer等人发表的基本方法。 (J. Bacteriol。> 124 :225-231,1975),我们已经能够从 Streptococcus ferus (以前是 Streptococcus mutans >亚种 ferus )通过遗传转化转化为血链球菌。在该系统中,隐性质粒的进入是间接选择的。这是通过转化脱氧核糖核酸混合物来实现的,其中隐性质粒脱氧核糖核酸相对于已知赋予红霉素抗性的质粒(pVA1)以大约10倍摩尔过量存在。在这种条件下,将5至10%的含pVA1抗性的红霉素转化体与隐性质粒脱氧核糖核酸共转化。 pVA1可以通过其 S的生长而选择性地消除。 sanguis 宿主菌株在42°C的温度下构建,可以构建带有和不带有 S的同基因菌株。 ferus 隐性质粒。此类菌株的比较生理研究未能揭示 S中任何质粒赋予的表型。通过此程序,我们已经能够物理分离两个小密码子(2.4×10 6 和2.8×10 6 道尔顿) > S。 。虽然这些质粒天然存在于单个 S中。 Ferus 宿主,它们能够在 S中彼此独立复制。限制性内切酶指纹图谱表明这些质粒不具有共同的血统。

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