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人类β-珠蛋白基因外显子1中5'剪接区域的G----C突变抑制前体mRNA剪接:一种β+地中海贫血的机制。

A 5' splice-region G----C mutation in exon 1 of the human beta-globin gene inhibits pre-mRNA splicing: a mechanism for beta+-thalassemia.

作者信息

Vidaud M, Gattoni R, Stevenin J, Vidaud D, Amselem S, Chibani J, Rosa J, Goossens M

机构信息

Institut National de la Santé et de la Recherche Médicale U.91, Hôpital Henri Mondor, Creteil, France.

出版信息

Proc Natl Acad Sci U S A. 1989 Feb;86(3):1041-5. doi: 10.1073/pnas.86.3.1041.

Abstract

We have characterized a Mediterranean beta-thalassemia allele containing a sequence change at codon 30 that alters both beta-globin pre-mRNA splicing and the structure of the hemoglobin product. Presumably, this G----C transversion at position -1 of intron 1 reduces severely the utilization of the normal 5' splice site since the level of the Arg----Thr mutant hemoglobin (designated hemoglobin Kairouan) found in the erythrocytes of the patient is very low (2% of total hemoglobin). Since no natural mutations of the guanine located at position -1 of the CAG/GTAAGT consensus sequence had been isolated previously, we investigated the role of this nucleotide in the constitution of an active 5' splice site by studying the splicing of the pre-mRNA in cell-free extracts. We demonstrate that correct splicing of the mutant pre-mRNA is 98% inhibited. Our results provide further insights into the mechanisms of pre-mRNA maturation by revealing that the last residue of the exon plays a role at least equivalent to that of the intron residue at position +5.

摘要

我们已鉴定出一种地中海β-地中海贫血等位基因,其密码子30处存在序列变化,这会改变β-珠蛋白前体mRNA的剪接以及血红蛋白产物的结构。据推测,内含子1第-1位的这种G→C颠换严重降低了正常5'剪接位点的利用率,因为在患者红细胞中发现的精氨酸→苏氨酸突变型血红蛋白(称为凯鲁万血红蛋白)水平非常低(占总血红蛋白的2%)。由于先前尚未分离到位于CAG/GTAAGT共有序列第-1位的鸟嘌呤的天然突变,我们通过研究无细胞提取物中前体mRNA的剪接,调查了该核苷酸在活性5'剪接位点构成中的作用。我们证明突变型前体mRNA的正确剪接受98%的抑制。我们的结果通过揭示外显子的最后一个残基发挥的作用至少与内含子第+5位残基的作用相当,为前体mRNA成熟机制提供了进一步的见解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cf01/286617/b11791ca1c3a/pnas00243-0296-a.jpg

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