2012
DOI: 10.1261/rna.033852.112
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Functional characterization of two paralogs that are novel RNA binding proteins influencing mitochondrial transcripts of Trypanosoma brucei

Abstract: A majority of Trypanosoma brucei proteins have unknown functions, a consequence of its independent evolutionary history within the order Kinetoplastida that allowed for the emergence of several unique biological properties. Among these is RNA editing, needed for expression of mitochondrial-encoded genes. The recently discovered mitochondrial RNA binding complex 1 (MRB1) is composed of proteins with several functions in processing organellar RNA. We characterize two MRB1 subunits, referred to herein as MRB8170 … Show more

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Cited by 40 publications
(100 citation statements)
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“…Taken together, these data indicate that MRB1 core integrity is dependent on subunits such as MRB8620 and MRB11870 , whereas the presence of the GAP1/2 heterotetramer is dispensable for its assembly or stability and even its association with TbRGG2. This finding plus the heterodispersion of the GAP1/2 subcomplex in density gradients (Acestor et al 2009;Hashimi et al 2009;Ammerman et al 2011Ammerman et al , 2012Kafková et al 2012;Aphasizheva et al 2014) and the association of GAP1/2 with REH2 (Madina et al 2014) or TbRGG3 (McAdams et al 2015 suggest that GAP1/2 interactions are not restricted to the MRB1 core and that the heterotetramer represents a functionally distinct entity.…”
Section: Discussionmentioning
confidence: 98%
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“…Taken together, these data indicate that MRB1 core integrity is dependent on subunits such as MRB8620 and MRB11870 , whereas the presence of the GAP1/2 heterotetramer is dispensable for its assembly or stability and even its association with TbRGG2. This finding plus the heterodispersion of the GAP1/2 subcomplex in density gradients (Acestor et al 2009;Hashimi et al 2009;Ammerman et al 2011Ammerman et al , 2012Kafková et al 2012;Aphasizheva et al 2014) and the association of GAP1/2 with REH2 (Madina et al 2014) or TbRGG3 (McAdams et al 2015 suggest that GAP1/2 interactions are not restricted to the MRB1 core and that the heterotetramer represents a functionally distinct entity.…”
Section: Discussionmentioning
confidence: 98%
“…MRB8620 has been shown to interact with the MRB1 core complex and the TbRGG2 subcomplex by yeast two-hybrid analysis and various tandem affinity purification (TAPs) of tagged MRB1 subunits Weng et al 2008;Hernandez et al 2010;Ammerman et al 2011Ammerman et al , 2012Kafková et al 2012). To confirm that MRB8620 is an integral component of the MRB1 complex, we analyzed proteins copurifying with the C-terminally PTP-tagged MRB8620 without nuclease treatment by LC-MS/MS mass spectroscopy.…”
Section: Mrb8620 Interacts With Other Mrb1 Subunitsmentioning
confidence: 99%
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“…The full ORF of HsLetm1 was PCR-amplified from cDNA (clone FLJ81927AAAF) supplied by the National Institute of Technology and Evaluation Biological Resource Center (Japan) using the forward primer TCAGATCTGCTCTTCACCTCTGCGA and reverse primer TCAGATCTTTGCTTCATGGC GTTGA and cloned into the pABPURO vector (43) via the underlined BglII restriction sites. We took advantage of every mRNA bearing a spliced leader RNA sequence by amplifying the 5Ј-end of Letm1 with the canonical spliced leader RNA forward primer and the reverse primer AGACATTAAACGGCCCTTCC, as described previously (44).…”
Section: Methodsmentioning
confidence: 99%