首页> 美国卫生研究院文献>Journal of Medical Genetics >Utilities for high throughput use of the single strand conformational polymorphism method: screening of 791 patients with familial hypercholesterolaemia for mutations in exon 3 of the low density lipoprotein receptor gene.
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Utilities for high throughput use of the single strand conformational polymorphism method: screening of 791 patients with familial hypercholesterolaemia for mutations in exon 3 of the low density lipoprotein receptor gene.

机译:单链构象多态性方法用于高通量的实用程序:筛选791名家族性高胆固醇血症患者低密度脂蛋白受体基因第3外显子的突变。

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摘要

We have modified several aspects of the single strand conformational polymorphism (SSCP) method to increase the speed with which the technique can be used for mutation detection. The methods attain high resolution of small mobility differences using long (30 cm) gels and use a modified polymerase reaction to maximise detection sensitivity using a minimised quantity of 32P. By using custom cut "sharktooth" combs (4.5 mm between teeth) as the slot formers, commercially available multichannel pipettes (9 mm tip to tip) can be used to load eight or 12 samples at a time from standard microtitre plates. PCR products that have been prepared and radiolabelled using simplified protocols are loaded on to the gel, and after a precalculated time of electrophoresis another set of samples can be loaded, either with combs moved across 2.25 mm or onto the same gel tracks. The run conditions are calculated so that there is no overlap between the bands produced by the two loadings, thus doubling the amount of information that can be gained from one gel. A computer program has been developed to solve equations to determine suitable timings for repetitive loadings. Finally, a modification of the gel pouring system is described so that two gels can be poured between three standard glass plates, with both gels run simultaneously. Of the order of 1000 PCR reactions can be prepared and analysed in 24 man hours using five 40 cm x 30 cm gel tanks. The application of these techniques is described to detect SSCPs in exon 3 of the low density lipoprotein receptor (LDLR) gene in 791 patients with familial hypercholesterolaemia (FH). Eight different SSCP patterns were seen, one of which was caused by the previously described E80K mutation, which was present in 11 patients (1.4%). In total, 32 patients (4%) were identified with exon 3 mutations.
机译:我们已经修改了单链构象多态性(SSCP)方法的几个方面,以提高该技术可用于突变检测的速度。该方法使用长(30 cm)凝胶可实现高分辨率的小迁移率差异,并使用改良的聚合酶反应以最小的32P量使检测灵敏度最大化。通过使用定制切割的“鲨齿”梳齿(齿间4.5 mm)作为开槽器,可以使用市售的多通道移液器(针尖到针尖9 mm)一次从标准微量滴定板中加载八或十二个样品。将使用简化方案制备并进行放射性标记的PCR产物上样到凝胶上,在经过预先计算的电泳时间后,可以上样另一组样品,既可以将梳子移动2.25毫米,也可以移动到相同的凝胶轨道上。计算运行条件时,两次加载产生的谱带之间不会重叠,因此可以从一种凝胶中获得的信息量加倍。已经开发了一种计算机程序来求解方程式,以确定重复加载的合适时间。最后,介绍了一种凝胶浇注系统的改进方案,可以将两种凝胶倒入三个标准玻璃板之间,并且两种凝胶同时运行。使用五个40 cm x 30 cm的凝胶槽,可以在24个工时内准备和分析1000次PCR反应。描述了这些技术的应用,以检测791例家族性高胆固醇血症(FH)患者的低密度脂蛋白受体(LDLR)基因外显子3中的SSCP。观察到八种不同的SSCP模式,其中一种是由先前描述的E80K突变引起的,该突变存在于11位患者中(1.4%)。总共鉴定出32位患者(4%)具有外显子3突变。

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