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烟粉虱及相关粉虱科的改进DNA条形码方法:通用及烟粉虱生物型特异性线粒体细胞色素c氧化酶I聚合酶链反应引物的开发

Improved DNA barcoding method for Bemisia tabaci and related Aleyrodidae: development of universal and Bemisia tabaci biotype-specific mitochondrial cytochrome c oxidase I polymerase chain reaction primers.

作者信息

Shatters Robert G, Powell Charles A, Boykin Laura M, Liansheng He, McKenzie C L

机构信息

United States Department of Agriculture, U.S. Horticultural Research Laboratory, Fort Pierce, FL 34945, USA.

出版信息

J Econ Entomol. 2009 Apr;102(2):750-8. doi: 10.1603/029.102.0236.

DOI:10.1603/029.102.0236
PMID:19449657
Abstract

Whiteflies, heteropterans in the family Aleyrodidae, are globally distributed and severe agricultural pests. The mitochondrial cytochrome c oxidase I (mtCOI) sequence has been used extensively in whitefly phylogenetic comparisons and in biotype identification of the agriculturally important Bemisia tabaci (Gennadius) whitefly. Because of the economic importance of several whitefly genera, and the invasive nature of the B and the Q biotypes of Bemisia tabaci, mtCOI sequence data are continually generated from sampled populations worldwide. Routine phylogenetic comparisons and biotype identification is done through amplification and sequencing of an approximately 800-bp mtCOI DNA fragment. Despite its routine use, published primers for amplification of this region are often inefficient for some B. tabaci biotypes and especially across whitefly species. Through new sequence generation and comparison to available whitefly mtCOI sequence data, a set of polymerase chain reaction (PCR) amplification primers (Btab-Uni primers) were identified that are more efficient at amplifying approximately 748 bp of the approximately 800-bp fragment currently used. These universal primers amplify an mtCOI fragment from numerous B. tabaci biotypes and whitefly genera by using a single amplification profile. Furthermore, mtCOI PCR primers specific for the B, Q, and New World biotypes of B. tabaci were designed that allow rapid discrimination among these biotypes. These primers produce a 478-, 405-, and 303-bp mtCOI fragment for the B, New World, and Q biotypes, respectively. By combining these primers and using rapid PCR and electrophoretic techniques, biotype determination can be made within 3 h for up to 96 samples at a time.

摘要

粉虱是粉虱科的半翅目昆虫,分布于全球,是严重的农业害虫。线粒体细胞色素c氧化酶I(mtCOI)序列已广泛用于粉虱系统发育比较以及对农业上重要的烟粉虱(Gennadius)粉虱的生物型鉴定。由于几种粉虱属具有经济重要性,以及烟粉虱B型和Q型具有入侵性,因此世界各地不断从采样种群中生成mtCOI序列数据。常规的系统发育比较和生物型鉴定是通过对大约800bp的mtCOI DNA片段进行扩增和测序来完成的。尽管该方法被常规使用,但已发表的用于扩增该区域的引物对某些烟粉虱生物型往往效率不高,尤其是在不同粉虱物种之间。通过新序列的生成并与现有的粉虱mtCOI序列数据进行比较,鉴定出了一组聚合酶链反应(PCR)扩增引物(Btab-Uni引物),它们在扩增目前使用的约800bp片段中的约748bp时效率更高。这些通用引物通过单一扩增程序从众多烟粉虱生物型和粉虱属中扩增出一个mtCOI片段。此外,还设计了针对烟粉虱B型、Q型和新大陆生物型的mtCOI PCR引物,可快速区分这些生物型。这些引物分别为B型、新大陆型和Q型生物型产生478bp、405bp和303bp的mtCOI片段。通过组合这些引物并使用快速PCR和电泳技术,一次最多可在3小时内对96个样品进行生物型测定。

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