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Binding of Recombinant but Not Endogenous Prion Protein to DNA Causes DNA Internalization and Expression in Mammalian Cells*

机译:重组但非内源性Pri蛋白与DNA结合导致DNA 哺乳动物的内在化和表达 细胞*

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摘要

Recombinant prion protein, rPrP, binds DNA. Both the KKRPK motif and the octapeptide repeat region of rPrP are essential for maximal binding. rPrP with pathogenic insertional mutations binds more DNA than wild-type rPrP. DNA promotes the aggregation of rPrP and protects its N terminus from proteinase K digestion. When rPrP is mixed with an expression plasmid and Ca2+, the rPrP·DNA complex is taken up by mammalian cells leading to gene expression. In the presence of Ca2+, rPrP by itself is also taken up by cells in a temperature- and pinocytosis-dependent manner. Cells do not take up rPrPΔKKRPK, which lacks the KKRPK motif. Thus, rPrP is the carrier for DNA and the KKRPK motif is essential for its uptake. When mixed with DNA, a pentapeptide KKRPK, but not KKKKK, is sufficient for DNA internalization and expression. In contrast, whereas the normal cellular prion protein, PrPC, on the cell surface can also internalize DNA, the imported DNA is not expressed. These findings may have relevance to the normal functions of PrPC and the pathogenic mechanisms of human prion disease.
机译:重组病毒蛋白rPrP与DNA结合。 KKRPK基序和rPrP的八肽重复区对于最大结合至关重要。具有致病性插入突变的rPrP与野生型rPrP结合的DNA更多。 DNA促进rPrP的聚集并保护其N末端免于蛋白酶K的消化。当rPrP与表达质粒和Ca2 +混合时,rPrP·DNA复合物被哺乳动物细胞吸收,导致基因表达。在存在Ca2 +的情况下,rPrP本身也被细胞以依赖温度和胞饮作用的方式摄取。细胞不吸收缺少KKRPK基序的rPrPΔKKRPK。因此,rPrP是DNA的载体,而KKRPK基序对于其摄取至关重要。当与DNA混合时,五肽KKRPK(而不是KKKKK)足以用于DNA内在化和表达。相反,尽管正常的细胞病毒蛋白PrPC在细胞表面也可以使DNA内在化,但导入的DNA不表达。这些发现可能与PrPC的正常功能和人类病毒病的致病机制有关。

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