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引用次数: 0
摘要
VLDL 受体的配体结合结构域包含八个不完全相似的重复序列。为了探讨每个重复序列对配体结合的贡献,研究人员利用 RT-PCR 技术从中国人的心肌中克隆了 VLDLR 的 cDNA。进一步构建了两个重组体,分别包含 VLDLR 的全长 cDNA 和缺少 1-5 重复序列的突变体。用两个重组体转染 CHO 细胞系。转染 pCD-VR 的 CHO 细胞可通过 RT-PCR 检测到 VLDLR 基因的表达。结合实验结果表明,转染 VLDL-R 全长 cDNA 的 CHO 细胞结合 DiI 标记的 beta-VLDL 的能力高于转染突变体的 CHO 细胞。我们的研究结果表明,人VLDL-R基因可在CHO细胞上有效表达,而删除重复序列1-5后,受体几乎失活。
The binding ability analysis of the normal VLDL receptor and its mutant.
The ligand-binding domain of VLDL receptor contains eight imperfectly similar repeats. To discuss the contribution of each repeat to ligand binding, the RT-PCR technique was used to clone the VLDLR-cDNA from the heart muscle of Chinese people. Two recombinants were further constructed, which contained the full-length cDNA of VLDLR and the mutant lacking repeats 1-5. CHO cell line was transfected with two recombinants. The expression of VLDLR gene could be detected by RT-PCR from the CHO cells transfected with pCD-VR. The results of binding experiments showed that the ability of the CHO cells transfected with the full-length cDNA of VLDL-R binding DiI-labeled beta-VLDL was higher than that of the CHO cells transfected with the mutant. Our findings indicated that human VLDL-R gene could be expressed effectively on CHO cells, and the receptor was almost inactivated when repeats 1-5 were deleted.
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