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RFLP analysis of mitochondrial DNA in two cytoplasmic male sterility systems (CMS-D2 and CMS-D8) of cotton

机译:棉花两个胞质雄性不育系统(CMS-D2和CMS-D8)中线粒体DNA的RFLP分析

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Cytoplasmic male sterility (CMS) in higher plants is a maternally inherited trait and CMS-associated genes are known to be located in the mitochondrial genome. However, CMS-inducing genes in CMS-D2 and CMS-D8 of Upland cotton (Gossypium hirsutum L., AD1) are currently unknown. The objective of this study was to identify potential candidate DNA or gene sequences for CMS-D2 and CMS-D8 through restriction fragment length polymorphism (RFLP) analysis. Seven mtDNA gene probes and five restriction enzymes were first used to compare D2 (from G. harknessii Brandegee) and AD1 cytoplasms. With cox1, cox2, and atp1 as probes, RFLP polymorphisms were detected with one or more restriction enzyme digestions. The most notable difference was an additional fragment in the normal AD1 cytoplasm detected by cox2 in digests of three enzymes, and by cox1 and atp1 in digests with PstI. The RFLP analysis was then conducted among CMS-D2, CMS-D8 (from G. trilobum (DC.) Skovst.), and AD1 cytoplasms. Two probes from maize, atp1 and atp6, detected polymorphism among the different cytoplasmic lines. However, no difference in RFLP patterns was noted between male sterile (A) and restorer (R) lines with the D2 or D8 cytoplasm, indicating that the presence of the D2 or D8 restorer gene does not affect mtDNA organization in Upland cotton. The results demonstrate that RFLP using atp1 and atp6 as probes can distinguish the three cytoplasms. The atp1 and atp6 in CMS-D8 and these two genes together with cox1 and cox2 in CMS-D2 could be the candidates of CMS-associated genes in the mitochondrial genome, providing information for further molecular studies and developing PCR-based markers for the CMS cytoplasms in breeding. This research represents the first work using RFLP to analyze the genetic basis of CMS in cotton.
机译:高等植物中的细胞质雄性不育(CMS)是母系遗传的性状,并且已知与CMS相关的基因位于线粒体基因组中。然而,目前尚不知道陆地棉(Gossypium hirsutum L.,AD1)的CMS-D2和CMS-D8中的CMS诱导基因。这项研究的目的是通过限制性片段长度多态性(RFLP)分析来识别CMS-D2和CMS-D8的潜在候选DNA或基因序列。首先使用七种mtDNA基因探针和五种限制酶来比较D2(来自G. harknessii Brandegee)和AD1细胞质。以cox1,cox2和atp1为探针,通过一种或多种限制酶消化检测到RFLP多态性。最显着的差异是正常AD1细胞质中的另外一个片段,由三种酶的消化物中的cox2以及由PstI消化的cox1和atp1检测到。然后在CMS-D2,CMS-D8(来自G. trilobum(DC。)Skovst。)和AD1细胞质中进行RFLP分析。来自玉米的两个探针atp1和atp6检测到不同细胞质系之间的多态性。然而,在具有D2或D8细胞质的雄性不育系(A)和恢复系(R)之间,没有发现RFLP模式的差异,这表明D2或D8恢复系基因的存在并不影响陆地棉的mtDNA组织。结果表明,使用atp1和atp6作为探针的RFLP可以区分三种细胞质。 CMS-D8中的atp1和atp6以及CMS-D2中的这两个基因以及cox1和cox2可能是线粒体基因组中CMS相关基因的候选基因,为进一步的分子研究和开发基于PCR的CMS标记提供信息繁殖中的细胞质。这项研究代表了使用RFLP分析棉花CMS遗传基础的第一项工作。

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