Mohan K S, Walia S K
Department of Biological Sciences, Oakland University, Rochester, MI 48309.
Can J Microbiol. 1994 Nov;40(11):969-73. doi: 10.1139/m94-154.
The soluble methane monooxygenase (sMMO) enzyme complex of methanotrophs cometabolizes haloaliphatic compounds such as trichloroethylene. Two 18-mer oligonucleotides as primary primers and a nested primer of the same length were selected to amplify specific DNA sequences of the sMMO gene cluster using polymerase chain reaction (PCR). Two DNA fragments of sizes 270 and 400 base pairs were obtained when purified DNA from the methanotroph Methylosinus trichosporium OB3b was used as template. The primers were specific for sMMO sequences of M. trichosporium, since none of the 13 bacterial isolates screened yielded the expected length of PCR-amplified DNA fragments. The detection limit of the PCR method was 5 x 10(2) cells of M. trichosporium. The sMMO sequences were successfully amplified in groundwater (containing native microbial population) when seeded with M. trichosporium, FP1 sense (5'-ATGTCCAGCGCTCATAAC-3'), RP1 antisense (5'-TCAGATGTCGGTCAGGGC-3'), FP2 sense nested (5'GCCATCATCGGTCAGGGC-3'), and FP2 sense nested (5'-GCCATCATCGAGGACATC-3').
甲烷营养菌的可溶性甲烷单加氧酶(sMMO)酶复合物可共代谢卤代脂肪族化合物,如三氯乙烯。选择两条18聚体寡核苷酸作为一级引物和一条相同长度的巢式引物,使用聚合酶链反应(PCR)扩增sMMO基因簇的特定DNA序列。当以甲烷营养菌 trichosporium OB3b的纯化DNA为模板时,获得了两条大小分别为270和400个碱基对的DNA片段。这些引物对 trichosporium的sMMO序列具有特异性,因为在筛选的13株细菌分离物中,没有一个产生预期长度的PCR扩增DNA片段。PCR方法的检测限为5×10²个 trichosporium细胞。当接种 trichosporium时,在地下水(含有天然微生物群落)中成功扩增了sMMO序列,并使用了FP1正义链(5'-ATGTCCAGCGCTCATAAC-3')、RP1反义链(5'-TCAGATGTCGGTCAGGGC-3')、FP2正义链巢式引物(5'GCCATCATCGGTCAGGGC-3')和FP2正义链巢式引物(5'-GCCATCATCGAGGACATC-3')。
