a la autoantigen homologue is required for the internal ribosome entry site mediated translation of giardiavirusla自身抗原同系物是所需的内部核糖体进入网站翻译giardiavirus介导的.pdfVIP
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a la autoantigen homologue is required for the internal ribosome entry site mediated translation of giardiavirusla自身抗原同系物是所需的内部核糖体进入网站翻译giardiavirus介导的
A La Autoantigen Homologue Is Required for the Internal
Ribosome Entry Site Mediated Translation of Giardiavirus
Srinivas Garlapati, Ashesh A. Saraiya, Ching C. Wang*
Department of Pharmaceutical Chemistry, University of California San Francisco, San Francisco, California, United States of America
Abstract
Translation of Giardiavirus (GLV) mRNA is initiated at an internal ribosome entry site (IRES) in the viral transcript. The IRES
localizes to a downstream portion of 59 untranslated region (UTR) and a part of the early downstream coding region of the
transcript. Recent studies indicated that the IRES does not require a pre-initiation complex to initiate translation but may
directly recruit the small ribosome subunit with the help of a number of trans-activating protein factors. A La autoantigen
homologue in the viral host Giardia lamblia, GlLa, was proposed as one of the potential trans-activating factors based on its
specific binding to GLV-IRES in vitro. In this study, we further elucidated the functional role of GlLa in GLV-IRES mediated
translation in Giardia by knocking down GlLa with antisense morpholino oligo, which resulted in a reduction of GLV-IRES
activity by 40%. An over-expression of GlLa in Giardia moderately stimulated GLV-IRES activity by 20%. A yeast inhibitory
RNA (IRNA), known to bind mammalian and yeast La autoantigen and inhibit Poliovirus and Hepatitis C virus IRES activities
in vitro and in vivo, was also found to bind to GlLa protein in vitro and inhibited GLV-IRES function in vivo. The C-terminal
domain of La autoantigen interferes with the dimerization of La and inhibits its function. An over-expression of the C-
terminal domain (200–348aa) of GlLa in Giardia showed a dominant-negative effect on GLV-IRES activity, suggesting a
potential inhibition of GlLa dimerization. HA tagged GlLa protein was detected mainly in the cy
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