首页> 美国卫生研究院文献>Journal of Virology >Molecular and biological properties of c-mil transducing retroviruses generated during passage of Rous-associated virus type 1 in chicken neuroretina cells.
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Molecular and biological properties of c-mil transducing retroviruses generated during passage of Rous-associated virus type 1 in chicken neuroretina cells.

机译:在鸡神经视网膜细胞中传递1型劳斯相关病毒的过程中产生的c-mil转导逆转录病毒的分子和生物学特性。

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摘要

IC1, IC2, and IC3 are novel c-mil transducing retroviruses generated during serial passaging of Rous-associated virus type 1 (RAV-1) in chicken embryo neuroretina cells. They were isolated by their ability to induce proliferation of these nondividing cells. IC2 and IC3 were generated during early passages of RAV-1 in neuroretina cells, whereas IC1 was isolated after six consecutive passages of virus supernatants. We sequenced the transduced genes and the mil-RAV-1 junctions of the three viruses. The 5' RAV-1-mil junction of IC2 and IC3 was formed by a splicing process between the RAV-1 leader sequence and exon 8 of the c-mil gene. The 5' end of IC1 resulted from homologous recombination between gag and mil sequences. Reconstitution experiments showed that serial passaging of IC2 in neuroretina cells also led to the formation of a gag-mil-containing retrovirus. Therefore, constitution of a U5-leader-delta c-mil-delta RAV-1-U3 virus represents early steps in c-mil transduction by RAV-1. This virus further recombined with RAV-1 to generate a gag-mil-containing virus. The three IC viruses transduced the serine/threonine kinase domain of the cellular gene. Hence, amino-terminal truncation is sufficient to activate the mitogenic property of c-mil. Comparison of the transforming properties of IC2 and IC1 showed that the transduced mil gene, expressed as a unique protein independent of gag sequences, was weakly transforming in avian cells. Acquisition of gag sequences by IC1 not only increased the rate of virus replication but also enhanced the transforming capacity of the virus.
机译:IC1,IC2和IC3是在鸡胚神经视网膜细胞中连续传递Rous相关病毒1型(RAV-1)时产生的新型c-mil转导逆转录病毒。通过它们诱导这些非分裂细胞增殖的能力将它们分离。 IC2和IC3是在RAV-1在神经视网膜细胞中早期传代过程中产生的,而IC1是在病毒上清液连续传代六次后分离出来的。我们对三种病毒的转导基因和mil-RAV-1接头进行了测序。 IC2和IC3的5'RAV-1-mil连接是通过RAV-1前导序列与c-mil基因的外显子8之间的剪接过程形成的。 IC1的5'端源于gag和mil序列之间的同源重组。重建实验表明,神经视网膜细胞中IC2的连续传代也导致含有gag-mil的逆转录病毒的形成。因此,U5-leader-delta c-mil-delta RAV-1-U3病毒的构成代表了RAV-1进行c-mil转导的早期步骤。该病毒进一步与RAV-1重组产生含gag-mil的病毒。三种IC病毒转导了细胞基因的丝氨酸/苏氨酸激酶结构域。因此,氨基末端的截短足以激活c-mil的有丝分裂特性。比较IC2和IC1的转化特性,发现转导的mil基因表达为独立于gag序列的独特蛋白质,在禽类细胞中的转化较弱。 IC1对gag序列的获取不仅增加了病毒复制的速度,而且还增强了病毒的转化能力。

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