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通过多重PCR鉴定与番茄黄化曲叶病和根结线虫抗性紧密连锁的标记

Identification of markers tightly linked to tomato yellow leaf curl disease and root-knot nematode resistance by multiplex PCR.

作者信息

Chen S X, Du J N, Hao L N, Wang C Y, Chen Q, Chang Y X

机构信息

College of Horticulture, Northwest A & F University, Key Laboratory of Horticultural Plant Germplasm Resources Utilization in Northwest, Yangling Shaanxi, P.R. China.

出版信息

Genet Mol Res. 2012 Aug 29;11(3):2917-28. doi: 10.4238/2012.July.10.4.

Abstract

Seven different commercial F₁ hybrids and two F₂ populations were evaluated by multiplex PCR to identify plants that are homozygous or heterozygous for Ty-1 and Mi, which confer resistance to tomato yellow leaf curl disease and root-knot nematode, respectively. The Ty-1 and Mi markers were amplified by PCR and identified by digestion of the amplicons with the TaqI enzyme. The hybrids E13 and 288 were found to be Ty/ty heterozygous plants with 398-, 303-, and 95-bp bands, and B08, 314, 198, and A10 were found to be ty/ty homozygous plants with a 398-bp band; whereas 098 did not give any PCR products. The hybrids E13 and 198 were found to be Mi/Mi homozygous plants with 570- and 180-bp bands, and 288 and A10 were found to be Mi/mi heterozygous plants, with 750-, 570- and 180-bp bands, and B08, 109 and 314 were found to be mi/mi homozygous plants with only a 750-bp band. We additionally developed a multiplex PCR technique for JB-1 and Mi, which confer resistance to tomato yellow leaf curl disease and root-knot nematode. The JB-1 marker identified the genotype of the Ty gene, and the plants that produced the 400-bp band were ty/ty homozygous plants, whereas the plants that produced 400- and 500-bp bands were resistant to tomato yellow leaf curl disease. We conclude that multiplex PCRs can be used to reproducibly and efficiently detect these resistance genes.

摘要

通过多重PCR对7种不同的商业F₁杂种和2个F₂群体进行评估,以鉴定对番茄黄化曲叶病和根结线虫具有抗性的Ty-1和Mi基因纯合或杂合的植株,其中Ty-1和Mi基因分别赋予对番茄黄化曲叶病和根结线虫的抗性。通过PCR扩增Ty-1和Mi标记,并使用TaqI酶消化扩增产物进行鉴定。发现杂种E13和288是具有398 bp、303 bp和95 bp条带的Ty/ty杂合植株,B08、314、198和A10是具有398 bp条带的ty/ty纯合植株;而098未产生任何PCR产物。发现杂种E13和198是具有570 bp和180 bp条带的Mi/Mi纯合植株,288和A10是具有750 bp、570 bp和180 bp条带的Mi/mi杂合植株,B08、109和314是仅具有750 bp条带的mi/mi纯合植株。我们还开发了一种针对JB-1和Mi的多重PCR技术,JB-1和Mi分别赋予对番茄黄化曲叶病和根结线虫的抗性。JB-1标记鉴定了Ty基因的基因型,产生400 bp条带的植株是ty/ty纯合植株,而产生400 bp和500 bp条带的植株对番茄黄化曲叶病具有抗性。我们得出结论,多重PCR可用于可重复且高效地检测这些抗性基因。

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