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用于检测β-珠蛋白基因的非同位素M13探针:在镰状细胞贫血诊断中的应用

Nonisotopic M13 probes for detecting the beta-globin gene: application to diagnosis of sickle cell anemia.

作者信息

Sheldon E, Kellogg D E, Levenson C, Bloch W, Aldwin L, Birch D, Goodson R, Sheridan P, Horn G, Watson R

出版信息

Clin Chem. 1987 Aug;33(8):1368-71.

PMID:3608154
Abstract

M13 DNA probes labeled with biotinylated psoralen and a streptavidin-horseradish peroxidase conjugate provide nonradioactive detection of the sickle cell and normal alleles of the beta-globin locus. The two biotinylated probes contain single-stranded sequences complementary to two different Sau3AI restriction fragments from the 5' region of the beta-globin gene and double-stranded M13 vector sequences. These probes are labeled with biotinylated psoralen photochemically linked to DNA. After hybridization, the presence of biotinylated probe bound to target DNA is detected in 3 h by using a streptavidin-horseradish peroxidase conjugate and the substrate, 3,3',5,5'-tetramethylbenzidine. Digestion of the normal (beta A) allele of the beta-globin gene with MstII (or isoschizomers) yields a 1.14-kb restriction fragment, while digestion of the mutant beta S allele yields a 1.34-kb fragment. These fragments can be resolved by gel electrophoresis and detected by Southern blot hybridization. The nonradioisotopic probe system can detect the beta-globin restriction fragment in as little as 0.5 microgram of human DNA and can distinguish heterozygotes (beta A beta S) from homozygotes (beta A beta A or beta S beta S) in 2.0 micrograms of human DNA.

摘要

用生物素化补骨脂素标记的M13 DNA探针和链霉亲和素 - 辣根过氧化物酶偶联物可对β - 珠蛋白基因座的镰状细胞和正常等位基因进行非放射性检测。这两种生物素化探针包含与β - 珠蛋白基因5'区域的两个不同Sau3AI限制性片段互补的单链序列以及双链M13载体序列。这些探针通过光化学方法将生物素化补骨脂素与DNA相连进行标记。杂交后,通过使用链霉亲和素 - 辣根过氧化物酶偶联物和底物3,3',5,5'-四甲基联苯胺,在3小时内检测到与靶DNA结合的生物素化探针的存在。用MstII(或同裂酶)消化β - 珠蛋白基因的正常(βA)等位基因会产生一个1.14 kb的限制性片段,而消化突变的βS等位基因会产生一个1.34 kb的片段。这些片段可通过凝胶电泳分离并通过Southern印迹杂交检测。这种非放射性探针系统在仅0.5微克的人类DNA中就能检测到β - 珠蛋白限制性片段,并且在2.0微克的人类DNA中能够区分杂合子(βAβS)和纯合子(βAβA或βSβS)。

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