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Implementation of two high through-put techniques in a novel application: detecting point mutations in large EMS mutated plant populations

机译:两种高通量技术在新应用中的实现:在大型EMS突变植物种群中检测点突变

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Background The establishment of mutant populations together with the strategies for targeted mutation detection has been applied successfully to a large number of organisms including many species in the plant kingdom. Considerable efforts have been invested into research on tomato as a model for berry-fruit plants. With the progress of the tomato sequencing project, reverse genetics becomes an obvious and achievable goal. Results Here we describe the treatment of Solanum lycopersicum seeds with 1% EMS and the development of a new mutated tomato population. To increase targeted mutant detection throughput an automated seed DNA extraction has been combined with novel mutation detection platforms for TILLING in plants. We have adapted two techniques used in human genetic diagnostics: Conformation Sensitive Capillary Electrophoresis (CSCE) and High Resolution DNA Melting Analysis (HRM) to mutation screening in DNA pools. Classical TILLING involves critical and time consuming steps such as endonuclease digestion reactions and gel electrophoresis runs. Using CSCE or HRM, the only step required is a simple PCR before either capillary electrophoresis or DNA melting curve analysis. Here we describe the development of a mutant tomato population, the setting up of two polymorphism detection platforms for plants and the results of the first screens as mutation density in the populations and estimation of the false-positives rate when using HRM to screen DNA pools. Conclusion These results demonstrate that CSCE and HRM are fast, affordable and sensitive techniques for mutation detection in DNA pools and therefore allow the rapid identification of new allelic variants in a mutant population. Results from the first screens indicate that the mutagen treatment has been effective with an average mutation detection rate per diploid genome of 1.36 mutation/kb/1000 lines.
机译:背景技术突变种群的建立以及针对性突变检测的策略已成功地应用于包括植物界中的许多物种在内的多种生物。已经将大量的精力投入到番茄研究中,将其作为浆果类植物的模型。随着番茄测序项目的进展,反向遗传学成为一个显而易见且可实现的目标。结果在这里,我们描述了用1%EMS处理茄子种子的方法以及一个新的突变番茄种群的发展。为了提高目标突变检测的通量,将自动种子DNA提取与新型突变检测平台结合在一起,用于植物的TILLING。我们将人类遗传学诊断中使用的两种技术进行了调整:构象敏感型毛细管电泳(CSCE)和高分辨率DNA熔解分析(HRM),以进行DNA池中的突变筛选。经典的填充涉及关键且耗时的步骤,例如核酸内切酶消化反应和凝胶电泳运行。使用CSCE或HRM,唯一需要的步骤是在毛细管电泳或DNA熔解曲线分析之前进行简单的PCR。在这里,我们描述了一个突变番茄种群的发展,两个植物多态性检测平台的建立以及作为群体中突变密度的第一个筛选结果以及使用HRM筛选DNA池时假阳性率的估计。结论这些结果表明CSCE和HRM是用于DNA池中突变检测的快速,可负担且灵敏的技术,因此可以快速鉴定突变群体中的新等位基因变体。最初筛选的结果表明,诱变剂处理有效,每个二倍体基因组的平均突变检测率为1.36突变/ kb / 1000株。

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