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Microsatellite primers for red drum (Sciaenops ocellatus)

机译:红鼓(Sciaenops ocellatus)的微卫星底漆

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摘要

In this note, we document polymerase-chain-reaction (PCR) primer pairs for 101 nuclear-encoded microsatellitesuddesigned and developed from a genomic library for red drum (Sciaenops ocellatus). Details of the genomic library construction, the sequencing of positive clones, primer design, and PCR protocols may be found in Karlsson et al. (2008). The 101 microsatellites (GENBA NK Accession NumbersudEU015882-EU015982) were amplified successfully and used to genotype 24 red drum obtained from Galveston Bay, Texas (Table 1). A total of 69 of the microsatellites had an uninterrupted (perfect) dinucleotide motif, and 30 had an imperfect dinucleotide motif; one microsatellite had anudimperfect tetranucleotide motif, and one had an imperfect and compound motif (Table 1 ). Sizes of the cloned alleles ranged from 84 to 252 base pairs. A ‘blast’ search of the GENBANK database indicated that all of the primers and the cloned alleles were unique (i.e., not duplicated).
机译:在本说明中,我们记录了从红鼓基因组(Sciaenops ocellatus)基因组文库中设计和开发的101种核编码微卫星的聚合酶链反应(PCR)引物对。基因组文库构建,阳性克隆测序,引物设计和PCR方案的详细信息,请参见Karlsson等。 (2008)。成功扩增了101个微卫星(GENBA NK登记号 udEU015882-EU015982),并用于对得克萨斯州加尔维斯顿湾的24个红鼓进行基因分型(表1)。共有69个微卫星具有不间断(完美)的二核苷酸基序,还有30个具有不完善的二核苷酸基序;一种微卫星具有不完美的四核苷酸基序,一种具有不完美的复合基序(表1)。克隆的等位基因的大小范围为84至252个碱基对。对GENBANK数据库的“爆炸”搜索表明,所有引物和克隆的等位基因都是唯一的(即,没有重复的)。

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