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Co-packaging of non-vector RNAs generates replication-defective retroviral vector particles: a novel approach for blocking retrovirus replication.

机译:非载体RNA的共同包装可产生复制缺陷型逆转录病毒载体颗粒:一种阻断逆转录病毒复制的新方法。

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摘要

A Moloney murine leukemia virus (MoMuLV)-derived packaging retroviral vector, pUCMoTN-PR3, was previously developed in which the packaging (psi) signal was cloned within the 5'-long terminal repeat (LTR) U3-r and U5 sequences. The MoTN-PR3 vector particles released from a transfected packaging cell line contain RNAs with r-psi-U5 sequences at the 5'-end and U3-r sequences at the 3'-end. Upon infection, these vector particles can efficiently transduce the neomycin phosphotransferase (neo) gene to the target cells. The structure of the proviral DNA synthesized in these cells was shown to contain modified 5'- and 3'-LTRs with U3-r-psi-U5 sequences, indicating that this vector can undergo reverse transcription and integration. Analysis of psi signal-containing RNAs revealed that in addition to vector RNA transcribed from the MoMuLV 5'-LTR promoter, readthrough neo RNA transcribed from the internal herpes simplex virus (HSV) thymidine kinase (tk) promoter and cellular RNAs transcribed from the MoMuLV 3'-LTR promoter are produced. Of these, the downstream cellular RNAs are also packaged within the vector particles. These vector particles containing the vector and non-vector RNAs carrying the MoMuLV psi signal are non-infectious. It is proposed that intracellular expression of packageable non-viral RNAs may represent an effective strategy for inhibiting animal and plant virus replication.
机译:先前开发了源自​​莫洛尼氏鼠白血病病毒(MoMuLV)的包装逆转录病毒载体pUCMoTN-PR3,其中包装(psi)信号被克隆在5'长的末端重复序列(LTR)U3-r和U5序列内。从转染的包装细胞系中释放的MoTN-PR3载体颗粒包含在5'端具有r-psi-U5序列,在3'端具有U3-r序列的RNA。感染后,这些载体颗粒可以有效地将新霉素磷酸转移酶(neo)基因转导至靶细胞。在这些细胞中合成的原病毒DNA的结构显示包含带有U3-r-psi-U5序列的修饰的5'-和3'-LTR,表明该载体可以进行逆转录和整合。对包含psi信号的RNA的分析表明,除了从MoMuLV 5'-LTR启动子转录的载体RNA之外,从内部单纯疱疹病毒(HSV)胸苷激酶(tk)启动子转录的通读新RNA和从MoMuLV转录的细胞RNA产生3'-LTR启动子。其中,下游细胞RNA也被包装在载体颗粒内。这些包含带有MoMuLV psi信号的载体和非载体RNA的载体颗粒是非传染性的。有人提出可包装的非病毒RNA的细胞内表达可能代表一种抑制动植物病毒复制的有效策略。

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