ARCD-1, an apobec-1-related cytidine deaminase, exerts  a dominant negative effect on C to U RNA editing

Anant, Shrikant; Mukhopadhyay, Debnath; Sankaranand, V.S.; Kennedy, Susan; Henderson, Jeffrey O.; Davidson, Nicholas O.

doi:10.1152/ajpcell.2001.281.6.c1904

Cited by 50 publications

(44 citation statements)

References 41 publications

(67 reference statements)

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“…Previous biochemical studies of mammalian Apobec2 proteins have questioned their catalytic activity (9 -11) and their ability to bind large polynucleotides (3,4). Here we show that Apobec2a,2b, like their mammalian orthologs, do not increase survival in bacterial mutagenesis assays.…”

Section: Discussionmentioning

confidence: 49%

“…Apobec2 was the second Apobec family member identified (2,3). Although its overexpression has been correlated with tumor formation, and its deletion correlated with perturbations in muscle development, retina regeneration, and left-right axis specification, the biochemical function of Apobec2 remains unknown (4 -8).…”

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confidence: 99%

“…Although its overexpression has been correlated with tumor formation, and its deletion correlated with perturbations in muscle development, retina regeneration, and left-right axis specification, the biochemical function of Apobec2 remains unknown (4 -8). Unlike other Apobecs, Apobec2 fails to induce cytosine deaminase-dependent mutations in bacterial and yeast-based mutagenesis assays (deamination of cytosine results in its conversion to uracil) (9 -11), and the ability of Apobec2 to bind polynucleotides is limited (3,4). Although biochemical data are lacking, prominent models of Apobec2 function include cytosine deaminase-dependent DNA demethylation (12,13) and C-to-U mRNA editing (5,6,8).…”

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confidence: 99%

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Zinc-binding Domain-dependent, Deaminase-independent Actions of Apolipoprotein B mRNA-editing Enzyme, Catalytic Polypeptide 2 (Apobec2), Mediate Its Effect on Zebrafish Retina Regeneration

Powell

Cornblath

Goldman

2014

Journal of Biological Chemistry

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Background:The mechanism by which Apobec2 stimulates retina regeneration remains unresolved. Results: Apobec2 lacks cytosine deaminase activity and interacts with proteins that regulate retina regeneration. Conclusion: Apobec2 subcellular localization is regulated by sumoylation and requires a zinc binding domain and protein interactions to regulate retina regeneration. Significance: This study delineates previously unidentified biochemical functions of Apobec2 proteins.

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Section: Discussionmentioning

confidence: 49%

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confidence: 99%

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confidence: 99%

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Zinc-binding Domain-dependent, Deaminase-independent Actions of Apolipoprotein B mRNA-editing Enzyme, Catalytic Polypeptide 2 (Apobec2), Mediate Its Effect on Zebrafish Retina Regeneration

Powell

Cornblath

Goldman

2014

Journal of Biological Chemistry

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“…It is possible that these proteins, like other Apobecs, catalytically edit RNAs, but it is also possible that they perform some function that is independent of a deaminase activity. Indeed, some have questioned whether Apobec2 proteins are catalytically active and whether they bind polynucleotides (36)(37)(38)(39). Further work is needed to shed light on the mechanism of these proteins.…”

Section: Discussionmentioning

confidence: 99%

Analysis of DNA methylation reveals a partial reprogramming of the Müller glia genome during retina regeneration

Powell

Grant

Cornblath

et al. 2013

Proc. Natl. Acad. Sci. U.S.A.

110

138

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Upon retinal injury, zebrafish Müller glia (MG) transition from a quiescent supportive cell to a progenitor cell (MGPC). This event is accompanied by the induction of key transcription and pluripotency factors. Because somatic cell reprogramming during induced pluripotent stem cell generation is accompanied by changes in DNA methylation, especially in pluripotency factor gene promoters, we were interested in determining whether DNA methylation changes also underlie MG reprogramming following retinal injury. Consistent with this idea, we found that genes encoding components of the DNA methylation/demethylation machinery were induced in MGPCs and that manipulating MGPC DNA methylation with 5-aza-2′-deoxycytidine altered their properties. A comprehensive analysis of the DNA methylation landscape as MG reprogram to MGPCs revealed that demethylation predominates at early times, whereas levels of de novo methylation increase at later times. We found that these changes in DNA methylation were largely independent of Apobec2 protein expression. A correlation between promoter DNA demethylation and injurydependent gene induction was noted. In contrast to induced pluripotent stem cell formation, we found that pluripotency factor gene promoters were already hypomethylated in quiescent MG and remained unchanged in MGPCs. Interestingly, these pluripotency factor promoters were also found to be hypomethylated in mouse MG. Our data identify a dynamic DNA methylation landscape as zebrafish MG transition to an MGPC and suggest that DNA methylation changes will complement other regulatory mechanisms to ensure gene expression programs controlling MG reprogramming are appropriately activated during retina regeneration.repair | multipotent | Ascl1 | bisulfite sequencing | DNA sequencing I nduced pluripotent stem cells (iPSCs) can be generated through the forced expression of pluripotency factor genes, such as Oct4, Klf4, Sox2, c-Myc, Lin28, and Nanog, which are normally expressed in embryonic stem cells (ESCs) (1, 2). Pluripotency factor gene expression in ESCs and iPSCs is associated with chromatin that is in an "open" accessible state, whereas their repression in somatic cells is associated with less accessible, condensed chromatin (3). DNA methylation has a significant impact on chromatin structure (3). DNA demethylation of pluripotency factor promoter regions is correlated with increased expression during iPSC formation (4, 5). Similar epigenetic changes are seen in other cellular reprogramming events such as nuclear transfer (6), heterokaryon formation (7), and carcinogenesis (8).Tissue regeneration provides another avenue to study cellular reprogramming. Unlike mammals, zebrafish can regenerate multiple tissues, including the retina. During zebrafish retina regeneration, Müller glia (MG) reprogram to generate progenitor cells (MGPCs) capable of replacing all lost neural cell types (9-12). The role that MG play during this regenerative event can be roughly divided into three phases: the replication-independent transition of MG to...

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“…The distance matrix was generated using the PROTDIST program, followed by the generation of a tree by the KITSCH programme, which was plotted using the DRAWTREE program [18].…”

Section: Phylogenetic Analysismentioning

confidence: 99%

Biochemical and molecular characterization of two cytidine deaminases in the nematode Caenorhabditis elegans

Thompson

Britton

Wheatley

et al. 2002

Biochemical Journal

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Two cytidine deaminases (CDDs) from the free-living nematode Caenorhabditis elegans have been cloned and characterized. Both Ce-CDD-1 and Ce-CDD-2 are authentic deaminases and both exhibit RNA-binding activity towards AU-rich templates. In order to study their temporal and spatial expression patterns in the worm, reporter gene constructs were made using approx. 2kb of upstream sequence. Transfection of C. elegans revealed that both genes localized to the cells of the intestine, although their temporal expression patterns were different. Expression of Ce-cdd-1 peaked in the early larval stages, whereas Ce-cdd-2 was expressed in all life cycle stages examined. RNA-interference (RNAi) assays were performed for both genes, either alone or in combination, but only cdd-2 RNAi produced a consistent visible phenotype. A proportion of eggs laid from these worms were swollen and distorted in shape.

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ARCD-1, an apobec-1-related cytidine deaminase, exerts a dominant negative effect on C to U RNA editing

Cited by 50 publications

References 41 publications

Zinc-binding Domain-dependent, Deaminase-independent Actions of Apolipoprotein B mRNA-editing Enzyme, Catalytic Polypeptide 2 (Apobec2), Mediate Its Effect on Zebrafish Retina Regeneration

Zinc-binding Domain-dependent, Deaminase-independent Actions of Apolipoprotein B mRNA-editing Enzyme, Catalytic Polypeptide 2 (Apobec2), Mediate Its Effect on Zebrafish Retina Regeneration

Analysis of DNA methylation reveals a partial reprogramming of the Müller glia genome during retina regeneration

Biochemical and molecular characterization of two cytidine deaminases in the nematode Caenorhabditis elegans

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