Ganguly A, Baldwin C T, Strobel D, Conway D, Horton W, Prockop D J
Department of Biochemistry and Molecular Biology, Thomas Jefferson University, Philadelphia, Pennsylvania 19107.
J Biol Chem. 1991 Jun 25;266(18):12035-40.
Cultured skin fibroblasts from a proband with osteogenesis imperfecta were found to synthesize normal and shortened alpha 2(I) chains of type I procollagen. A cDNA library was prepared using mRNA isolated from the proband's fibroblasts. Partial nucleotide sequencing of five clones demonstrated that two clones lacked the 54 base pairs (bp) of coding sequences found in exon 33 of the pro-alpha 2(I) gene (COL1A2). To reduce the amount of nucleotide sequencing required, heteroduplexes were prepared from two of the clones, one normal and the other lacking exon 33, and reacted with a water-soluble carbodiimide under conditions in which nonbase-paired G and T nucleotides are specifically modified by the reagent. Analysis of the heteroduplexes by immunoelectron microscopy suggested that the sequence variation near the codons of exon 33 was the only sequence difference in the cDNA clones. Amplification of cDNA from the proband by polymerase chain reaction gave products of two sizes, one of the expected size for the normal sequence and the other of the expected size for a product lacking the 54 bp in exon 33. To define the mutation in genomic DNA, a 1.6-kilobase region spanning exons 32 and 34 was amplified by the polymerase chain reaction and DNA heteroduplexes were prepared from the products. The heteroduplexes were treated with a water-soluble carbodiimide and then used as templates for primer extension under conditions in which extension terminates at the site of a carbodiimide-modified base. The results suggested a mismatch near the exon-intron boundary of exon 33 and a second mismatch near the 3' end of intron 33. Nucleotide sequencing of the polymerase chain reaction products revealed a single-base substitution in one allele that changed the moderately conserved G at position +5 of the 5' splice site of intron 33 to an A. In addition, there was an apparently neutral single-base substitution that placed both a G and T at position +661 of intron 33. The results provide only the third example of a mutation in the G at the +5 position of an intron that causes aberrant RNA splicing. Also, the results demonstrate that use of techniques involving carbodiimide modification of DNA heteroduplexes can reduce the amount of nucleotide sequencing necessary to define mutations in large and complex genes.
在一名成骨不全症先证者的培养皮肤成纤维细胞中,发现其能合成正常和缩短的I型前胶原α2(I)链。使用从先证者的成纤维细胞中分离出的mRNA制备了一个cDNA文库。对五个克隆进行部分核苷酸测序表明,两个克隆缺少在前α2(I)基因(COL1A2)第33外显子中发现的54个碱基对(bp)的编码序列。为了减少所需的核苷酸测序量,从两个克隆(一个正常,另一个缺少第33外显子)制备了异源双链体,并在非碱基配对的G和T核苷酸被该试剂特异性修饰的条件下与水溶性碳二亚胺反应。通过免疫电子显微镜对异源双链体进行分析表明,第33外显子密码子附近的序列变异是cDNA克隆中唯一的序列差异。通过聚合酶链反应从先证者的cDNA中扩增得到两种大小的产物,一种是正常序列预期大小的产物,另一种是缺少第33外显子中54 bp的产物预期大小的产物。为了确定基因组DNA中的突变,通过聚合酶链反应扩增了跨越第32和34外显子的1.6千碱基区域,并从产物中制备了DNA异源双链体。将异源双链体用水溶性碳二亚胺处理,然后在延伸终止于碳二亚胺修饰碱基位点的条件下用作引物延伸的模板。结果表明在第33外显子的外显子 - 内含子边界附近存在错配,在第33内含子的3'端附近存在第二个错配。对聚合酶链反应产物进行核苷酸测序揭示了一个等位基因中的单碱基替换,该替换将第33内含子5'剪接位点 +5位置的中度保守的G变为A。此外,存在一个明显中性的单碱基替换,使得第33内含子 +661位置同时出现G和T。这些结果仅提供了内含子 +5位置的G发生突变导致异常RNA剪接的第三个例子。此外,结果表明使用涉及DNA异源双链体碳二亚胺修饰的技术可以减少确定大型复杂基因中突变所需的核苷酸测序量。
