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甲状旁腺激素样蛋白:人类癌细胞系中的替代性信使核糖核酸剪接途径

Parathyroid hormone-like protein: alternative messenger RNA splicing pathways in human cancer cell lines.

作者信息

Brandt D W, Wachsman W, Deftos L J

机构信息

Department of Medicine, University of California, San Diego.

出版信息

Cancer Res. 1994 Feb 1;54(3):850-3.

PMID:8306349
Abstract

Parathyroid hormone-like protein (PLP) is expressed in a wide variety of cancers and exerts diverse biological effects in addition to hypercalcemia. We studied the expression of the gene for PLP in cancer cell lines derived from different tissues that produce PLP. We used the polymerase chain reaction to evaluate the PLP mRNA species produced in these various cell lines by differential transcription initiation and alternative splicing pathways. A series of exon-specific oligonucleotide primers that hybridize to DNA sequences adjacent to exon-intron splice junctions throughout the PLP gene were designed. These primers were used to evaluate steady state levels of PLP mRNA species. Our analysis with promoter-specific primers demonstrated expression from all three putative transcription start sites of PLP, designated P1, P2, and P3. P2-initiated transcripts were present in all of the cell lines, whereas the presence of P1- and P3-initiated messages were cell line specific. Our analysis with carboxy-terminal coding-specific primers demonstrated the utilization of the alternative splicing pathways that produce all three mature PLP polypeptides, PLP-139, -1-173, and -1-141. The 1-139 mRNA species was found in all of the cell lines, whereas the 1-141 and 1-173 mRNA species were cell line specific. These studies demonstrate the prevalence of the P2-initiated mRNA and the PLP1-139 alternative splicing pathway in the tumor cell lines studied and suggest that other pathways of PLP gene expression may be regulated in a cell line-dependent manner. The particular form of PLP expressed by a given cell can influence its biological effects.

摘要

甲状旁腺激素样蛋白(PLP)在多种癌症中表达,除导致高钙血症外还发挥多种生物学作用。我们研究了来自不同产生PLP组织的癌细胞系中PLP基因的表达情况。我们使用聚合酶链反应,通过差异转录起始和可变剪接途径评估这些不同细胞系中产生的PLP mRNA种类。设计了一系列与PLP基因中外显子-内含子剪接连接处相邻的DNA序列杂交的外显子特异性寡核苷酸引物。这些引物用于评估PLP mRNA种类的稳态水平。我们用启动子特异性引物进行的分析表明,PLP的所有三个推定转录起始位点(分别命名为P1、P2和P3)均有表达。P2起始的转录本存在于所有细胞系中,而P1和P3起始的信息则具有细胞系特异性。我们用羧基末端编码特异性引物进行的分析表明,可变剪接途径产生了所有三种成熟的PLP多肽,即PLP-139、-1-173和-1-141。1-139 mRNA种类存在于所有细胞系中,而1-141和1-173 mRNA种类具有细胞系特异性。这些研究表明,在所研究的肿瘤细胞系中,P2起始的mRNA和PLP1-139可变剪接途径普遍存在,并提示PLP基因表达的其他途径可能以细胞系依赖性方式受到调控。特定细胞表达的PLP特定形式可影响其生物学作用。

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