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乳酸乳球菌基因组DNA的克隆,该DNA可恢复噬菌体对一种不寻常的抗噬菌体sk1突变体的敏感性。

Cloning of genomic DNA of Lactococcus lactis that restores phage sensitivity to an unusual bacteriophage sk1-resistant mutant.

作者信息

Kraus J, Geller B L

机构信息

Department of Microbiology, Oregon State University, Corvallis, Oregon 97331-3804, USA.

出版信息

Appl Environ Microbiol. 2001 Feb;67(2):791-8. doi: 10.1128/AEM.67.2.791-798.2001.

Abstract

An unusual, spontaneous, phage sk1-resistant mutant (RMSK1/1) of Lactococcus lactis C2 apparently blocks phage DNA entry into the host. Although no visible plaques formed on RMSK1/1, this host propagated phage at a reduced efficiency. This was evident from center-of-infection experiments, which showed that 21% of infected RMSK1/1 formed plaques when plated on its phage-sensitive parental strain, C2. Moreover, viable cell counts 0 and 4 h after infection were not significantly different from those of an uninfected culture. Further characterization showed that phage adsorption was normal, but burst size was reduced fivefold and the latent period was increased from 28.5 to 36 min. RMSK1/1 was resistant to other, but not all, similar phages. Phage sensitivity was restored to RMSK1/1 by transformation with a cloned DNA fragment from a genomic library of a phage-sensitive strain. Characterization of the DNA that restored phage sensitivity revealed an open reading frame with similarity to sequences encoding lysozymes (beta-1,4-N-acetylmuramidase) and lysins from various bacteria, a fungus, and phages of Lactobacillus and Streptococcus and also revealed DNA homologous to noncoding sequences of temperate phage of L. lactis, DNA similar to a region of phage sk1, a gene with similarity to tRNA genes, a prophage attachment site, and open reading frames with similarities to sun and to sequences encoding phosphoprotein phosphatases and protein kinases. Mutational analyses of the cloned DNA showed that the region of homology with lactococcal temperate phage was responsible for restoring the phage-sensitive phenotype. The region of homology with DNA of lactococcal temperate phage was similar to DNA from a previously characterized lactococcal phage that suppresses an abortive infection mechanism of phage resistance. The region of homology with lactococcal temperate phage was deleted from a phage-sensitive strain, but the strain was not phage resistant. The results suggest that the cloned DNA with homology to lactococcal temperate phage was not mutated in the phage-resistant strain. The cloned DNA apparently suppressed the mechanism of resistance, and it may do so by mimicking a region of phage DNA that interacts with components of the resistance mechanism.

摘要

乳酸乳球菌C2的一种罕见的、自发的、抗噬菌体sk1的突变体(RMSK1/1)显然能阻止噬菌体DNA进入宿主细胞。虽然在RMSK1/1上未形成可见噬菌斑,但该宿主能以较低效率繁殖噬菌体。这在感染中心实验中很明显,该实验表明,当将感染后的RMSK1/1接种在其噬菌体敏感的亲本菌株C2上时,21%的RMSK1/1形成了噬菌斑。此外,感染后0小时和4小时的活细胞计数与未感染培养物的活细胞计数没有显著差异。进一步的特性分析表明,噬菌体吸附正常,但裂解量减少了五倍,潜伏期从28.5分钟增加到36分钟。RMSK1/1对其他一些但并非所有相似噬菌体具有抗性。通过用来自噬菌体敏感菌株基因组文库的克隆DNA片段转化,RMSK1/1恢复了噬菌体敏感性。对恢复噬菌体敏感性的DNA的特性分析揭示了一个开放阅读框,其与编码各种细菌、一种真菌以及乳酸杆菌和链球菌噬菌体的溶菌酶(β-1,4-N-乙酰胞壁酸酶)和溶素的序列相似,还揭示了与乳酸乳球菌温和噬菌体非编码序列同源的DNA、与噬菌体sk1一个区域相似的DNA、一个与tRNA基因相似的基因、一个原噬菌体附着位点以及与sun以及编码磷蛋白磷酸酶和蛋白激酶的序列相似的开放阅读框。对克隆DNA的突变分析表明,与乳酸乳球菌温和噬菌体的同源区域负责恢复噬菌体敏感表型。与乳酸乳球菌温和噬菌体DNA的同源区域与先前表征的一种抑制噬菌体抗性流产感染机制的乳酸乳球菌噬菌体的DNA相似。从噬菌体敏感菌株中删除了与乳酸乳球菌温和噬菌体同源的区域,但该菌株对噬菌体不具有抗性。结果表明,与乳酸乳球菌温和噬菌体同源的克隆DNA在噬菌体抗性菌株中未发生突变。克隆DNA显然抑制了抗性机制,它可能是通过模拟与抗性机制成分相互作用的噬菌体DNA区域来实现的。

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