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用于鉴定啤酒厂分离的片球菌的核糖体印记法和16S rRNA基因测序

Riboprinting and 16S rRNA gene sequencing for identification of brewery Pediococcus isolates.

作者信息

Barney M, Volgyi A, Navarro A, Ryder D

机构信息

Miller Brewing Company, Milwaukee, Wisconsin 53201, USA.

出版信息

Appl Environ Microbiol. 2001 Feb;67(2):553-60. doi: 10.1128/AEM.67.2.553-560.2001.

Abstract

A total of 46 brewery and 15 ATCC Pediococcus isolates were ribotyped using a Qualicon RiboPrinter. Of these, 41 isolates were identified as Pediococcus damnosus using EcoRI digestion. Three ATCC reference strains had patterns similar to each other and matched 17 of the brewery isolates. Six other brewing isolates were similar to ATCC 25249. The other 18 P. damnosus brewery isolates had unique patterns. Of the remaining brewing isolates, one was identified as P. parvulus, two were identified as P. acidilactici, and two were identified as unique Pediococcus species. The use of alternate restriction endonucleases indicated that PstI and PvuII could further differentiate some strains having identical EcoRI profiles. An acid-resistant P. damnosus isolate could be distinguished from non-acid-resistant varieties of the same species using PstI instead of EcoRI. 16S rRNA gene sequence analysis was compared to riboprinting for identifying pediococci. The complete 16S rRNA gene was PCR amplified and sequenced from seven brewery isolates and three ATCC references with distinctive riboprint patterns. The 16S rRNA gene sequences from six different brewery P. damnosus isolates were homologous with a high degree of similarity to the GenBank reference strain but were identical to each other and one ATCC strain with the exception of 1 bp in one strain. A slime-producing, beer spoilage isolate had 16S rRNA gene sequence homology to the P. acidilactici reference strain, in agreement with the riboprint data. Although 16S rRNA gene sequencing correctly identified the genus and species of the test Pediococcus isolates, riboprinting proved to be a better method for subspecies differentiation.

摘要

使用Qualicon RiboPrinter对总共46株啤酒厂分离株和15株ATCC片球菌分离株进行了核糖体分型。其中,41株分离株经EcoRI酶切鉴定为有害片球菌。三株ATCC参考菌株的图谱彼此相似,与17株啤酒厂分离株匹配。另外6株啤酒厂分离株与ATCC 25249相似。其余18株有害片球菌啤酒厂分离株具有独特的图谱。在其余的啤酒厂分离株中,一株被鉴定为微小片球菌,两株被鉴定为嗜酸片球菌,两株被鉴定为独特的片球菌物种。使用替代限制性内切酶表明,PstI和PvuII可以进一步区分一些具有相同EcoRI图谱的菌株。使用PstI而非EcoRI可以将一株耐酸的有害片球菌分离株与同一物种的非耐酸变种区分开来。将16S rRNA基因序列分析与核糖体分型用于鉴定片球菌。从七株具有独特核糖体分型图谱的啤酒厂分离株和三株ATCC参考菌株中PCR扩增并测序了完整的16S rRNA基因。来自六个不同啤酒厂有害片球菌分离株的16S rRNA基因序列与GenBank参考菌株具有高度同源性,但彼此相同,并且与一株ATCC菌株相同,只有一株中有1个碱基对不同。一株产黏液的啤酒腐败分离株的16S rRNA基因序列与嗜酸片球菌参考菌株具有同源性,这与核糖体分型数据一致。虽然16S rRNA基因测序正确鉴定了测试片球菌分离株的属和种,但核糖体分型被证明是一种更好的亚种区分方法。

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