Le Loir Y, Gruss A, Ehrlich S D, Langella P
Laboratorie de Génétique Microbienne, Institut National de la Recherche Agronomique, Jouy en Josas, France.
J Bacteriol. 1994 Aug;176(16):5135-9. doi: 10.1128/jb.176.16.5135-5139.1994.
A system for direct screening of recombinant clones in Lactococcus lactis, based on secretion of the staphylococcal nuclease (SNase) in the organism, was developed. The nuc gene (encoding SNase) was cloned on both rolling-circle and theta-replicating plasmids. L. lactis strains containing these nuc+ plasmids secrete SNase and are readily detectable by a simple plate test. A multicloning site (MCS) was introduced just after the cleavage site between leader peptide and the mature SNase, without affecting nuclease activity. Cloning foreign DNA fragments into any site of the MCS interrupts nuc and thus results in nuc mutant clones which are easily distinguished fron nuc+ clones on plates. The utility of this system for L. lactis was demonstrated by cloning an antibiotic resistance marker and Escherichia coli chromosomal DNA fragments into the MCS of the nucMCS cassette. Both cloning vectors containing the nucMCS cassette were also introduced into Streptococcus salivarius subsp. thermophilus, in which direct screening of nuc mutant recombinant clones was also achieved. The potential uses of nuc as a secretion reporter system are discussed.
开发了一种基于在乳酸乳球菌中分泌葡萄球菌核酸酶(SNase)来直接筛选重组克隆的系统。核酸酶基因(编码SNase)被克隆到滚环复制质粒和θ复制质粒上。含有这些nuc⁺质粒的乳酸乳球菌菌株分泌SNase,通过简单的平板试验即可轻松检测到。在引导肽和成熟SNase之间的切割位点之后引入了一个多克隆位点(MCS),而不影响核酸酶活性。将外源DNA片段克隆到MCS的任何位点会中断nuc,从而产生nuc突变体克隆,这些克隆在平板上很容易与nuc⁺克隆区分开来。通过将抗生素抗性标记和大肠杆菌染色体DNA片段克隆到nucMCS盒的MCS中,证明了该系统对乳酸乳球菌的实用性。含有nucMCS盒的两种克隆载体也被引入到嗜热唾液链球菌中,在该菌中也实现了对nuc突变体重组克隆的直接筛选。讨论了nuc作为分泌报告系统的潜在用途。