Your search keyword '"Cytidine Deaminase isolation & purification"' showing total 12 results

1. REG-γ associates with and modulates the abundance of nuclear activation-induced deaminase.

Author

Uchimura Y, Barton LF, Rada C, and Neuberger MS

Subjects

B-Lymphocytes cytology, Blotting, Western, Cell Line, Cytidine Deaminase isolation & purification, Humans, Immunoglobulin Class Switching physiology, Immunoprecipitation, Mass Spectrometry, Microscopy, Fluorescence, AICDA (Activation-Induced Cytidine Deaminase), Autoantigens metabolism, B-Lymphocytes metabolism, Cell Nucleus metabolism, Cytidine Deaminase metabolism, Proteasome Endopeptidase Complex metabolism

Abstract

Activation-induced deaminase (AID) acts on the immunoglobulin loci in activated B lymphocytes to initiate antibody gene diversification. The abundance of AID in the nucleus appears tightly regulated, with most nuclear AID being either degraded or exported back to the cytoplasm. To gain insight into the mechanisms regulating nuclear AID, we screened for proteins interacting specifically with it. We found that REG-γ, a protein implicated in ubiquitin- and ATP-independent protein degradation, interacts in high stoichiometry with overexpressed nuclear AID as well as with endogenous AID in B cells. REG-γ deficiency results in increased AID accumulation and increased immunoglobulin class switching. A stable stoichiometric AID-REG-γ complex can be recapitulated in co-transformed bacteria, and REG-γ accelerates proteasomal degradation of AID in in vitro assays. Thus, REG-γ interacts, likely directly, with nuclear AID and modulates the abundance of this antibody-diversifying but potentially oncogenic enzyme.

Published

2011

2. Crystal structure of the anti-viral APOBEC3G catalytic domain and functional implications.

Author

Holden LG, Prochnow C, Chang YP, Bransteitter R, Chelico L, Sen U, Stevens RC, Goodman MF, and Chen XS

Subjects

APOBEC Deaminases, APOBEC-3G Deaminase, Antiviral Agents, Crystallography, X-Ray, Cytidine Deaminase genetics, Cytidine Deaminase isolation & purification, DNA, Single-Stranded metabolism, Escherichia coli, Humans, Models, Molecular, Muscle Proteins chemistry, Mutant Proteins chemistry, Mutant Proteins genetics, Mutant Proteins metabolism, Mutation, Nuclear Magnetic Resonance, Biomolecular, Protein Structure, Secondary, Structural Homology, Protein, Structure-Activity Relationship, Substrate Specificity, Catalytic Domain, Cytidine Deaminase chemistry, Cytidine Deaminase metabolism

Abstract

The APOBEC family members are involved in diverse biological functions. APOBEC3G restricts the replication of human immunodeficiency virus (HIV), hepatitis B virus and retroelements by cytidine deamination on single-stranded DNA or by RNA binding. Here we report the high-resolution crystal structure of the carboxy-terminal deaminase domain of APOBEC3G (APOBEC3G-CD2) purified from Escherichia coli. The APOBEC3G-CD2 structure has a five-stranded beta-sheet core that is common to all known deaminase structures and closely resembles the structure of another APOBEC protein, APOBEC2 (ref. 5). A comparison of APOBEC3G-CD2 with other deaminase structures shows a structural conservation of the active-site loops that are directly involved in substrate binding. In the X-ray structure, these APOBEC3G active-site loops form a continuous 'substrate groove' around the active centre. The orientation of this putative substrate groove differs markedly (by 90 degrees) from the groove predicted by the NMR structure. We have introduced mutations around the groove, and have identified residues involved in substrate specificity, single-stranded DNA binding and deaminase activity. These results provide a basis for understanding the underlying mechanisms of substrate specificity for the APOBEC family.

Published

2008

3. Metabolic regulation of apoB mRNA editing is associated with phosphorylation of APOBEC-1 complementation factor.

Author

Lehmann DM, Galloway CA, Sowden MP, and Smith HC

Subjects

APOBEC-1 Deaminase, Animals, Apolipoproteins B metabolism, Cell Line, Cell Nucleus chemistry, Cell Nucleus enzymology, Cells, Cultured, Cytidine Deaminase isolation & purification, Enzyme Inhibitors pharmacology, Heterogeneous-Nuclear Ribonucleoproteins isolation & purification, Liver metabolism, Male, Phosphoprotein Phosphatases antagonists & inhibitors, Phosphoproteins isolation & purification, Phosphoproteins metabolism, Phosphorylation, RNA, Messenger metabolism, Rats, Rats, Sprague-Dawley, Apolipoproteins B genetics, Heterogeneous-Nuclear Ribonucleoproteins metabolism, RNA Editing drug effects

Abstract

Apolipoprotein B (apoB) mRNA editing is a nuclear event that minimally requires the RNA substrate, APOBEC-1 and APOBEC-1 Complementation Factor (ACF). The co-localization of these macro-molecules within the nucleus and the modulation of hepatic apoB mRNA editing activity have been described following a variety of metabolic perturbations, but the mechanism that regulates editosome assembly is unknown. APOBEC-1 was effectively co-immunoprecipitated with ACF from nuclear, but not cytoplasmic extracts. Moreover, alkaline phosphatase treatment of nuclear extracts reduced the amount of APOBEC-1 co-immunoprecipitated with ACF and inhibited in vitro editing activity. Ethanol stimulated apoB mRNA editing was associated with a 2- to 3-fold increase in ACF phosphorylation relative to that in control primary hepatocytes. Significantly, phosphorylated ACF was restricted to nuclear extracts where it co-sedimented with 27S editing competent complexes. Two-dimensional phosphoamino acid analysis of ACF immunopurified from hepatocyte nuclear extracts demonstrated phosphorylation of serine residues that was increased by ethanol treatment. Inhibition of protein phosphatase I, but not PPIIA or IIB, stimulated apoB mRNA editing activity coincident with enhanced ACF phosphorylation in vivo. These data demonstrate that ACF is a metabolically regulated phosphoprotein and suggest that this post-translational modification increases hepatic apoB mRNA editing activity by enhancing ACF nuclear localization/retention, facilitating the interaction of ACF with APOBEC-1 and thereby increasing the probability of editosome assembly and activity.

Published

2006

4. Activation-induced deaminase cloning, localization, and protein extraction from young VH-mutant rabbit appendix.

Author

Yang G, Obiakor H, Sinha RK, Newman BA, Hood BL, Conrads TP, Veenstra TD, and Mage RG

Subjects

Amino Acid Sequence, Animals, Base Sequence, Blotting, Western, Cell Division physiology, Chickens, Cytidine Deaminase isolation & purification, Fluorescent Antibody Technique, Humans, Immunohistochemistry, Mice, Molecular Sequence Data, Rabbits, Sequence Alignment, AICDA (Activation-Induced Cytidine Deaminase), Appendix enzymology, Cytidine Deaminase genetics, Cytidine Deaminase metabolism, Immunoglobulin Heavy Chains genetics, Immunoglobulin Variable Region genetics, Mutation

Abstract

Studies in mouse, human, and chicken suggest that activation-induced deaminase (AID) is involved in three known processes leading to antibody diversification: somatic hypermutation, gene conversion, and class-switch recombination. Developing rabbit appendix provides a particularly good site for studying all three of these B cell maturation events. We report here successful cloning of rabbit AID and isolation of AID protein from rabbit appendix-cell nuclear and cytoplasmic extracts. We succeeded in identifying and locating AID protein in cells by immunohistochemical and immunofluorescent staining techniques and examined colocalization of AID and other molecules important for Ab diversification. This report extends our knowledge about AID to a mammalian species that uses gene conversion to diversify rearranged Ig genes. Although much work remains to understand fully the mechanism of action of AID and its association with other cellular components, the rabbit system now offers a particularly useful model for future studies of these dynamics.

Published

2005

5. Isoenzymatic forms of human cytidine deaminase.

Author

Vincenzetti S, Mariani PL, Cammertoni N, Polzonetti V, Natalini P, Quadrini B, Volpini R, and Vita A

Subjects

Anion Exchange Resins pharmacology, Chromatography, Chromatography, Gel, Chromatography, Ion Exchange, Cloning, Molecular, Codon, DNA, Complementary metabolism, Escherichia coli metabolism, Humans, Isoelectric Focusing, Kinetics, Placenta enzymology, Protein Engineering methods, Protein Isoforms, Recombinant Proteins chemistry, Resins, Synthetic, Sodium Dodecyl Sulfate chemistry, Cytidine Deaminase chemistry, Cytidine Deaminase isolation & purification

Abstract

Cytidine deaminase (CDA) purified from human placenta revealed the presence of five isoenzymatic forms that differ only in their isoelectric point. Since human cytidine deaminase exists in two variants (CDA 1 and CDA 2) with a non-conservative amino acid substitution at codon 27, in this work we demonstrate that these two variants may combine together in vitro, giving five CDA isoforms as observed in vivo from human placenta. For this purpose, each of the two forms of CDA was purified close to homogeneity and dissociated into monomers in the presence of a small amount of sodium dodecyl sulfate as a dissociating agent. The monomers were mixed together and subjected to anion-exchange chromatography and to chromatofocusing analysis in order to visualize the formation of the five isoforms. Furthermore, for both CDA 1 and CDA 2 some substrates and inhibitors of CDA were assayed, with the aim of demonstrating different kinetic behavior between the two natural variants.

Published

2004

6. AID: how does it aid antibody diversity?

Author

Honjo T, Muramatsu M, and Fagarasan S

Subjects

Animals, B-Lymphocytes immunology, B-Lymphocytes metabolism, Cytidine Deaminase chemistry, Cytidine Deaminase genetics, Cytidine Deaminase isolation & purification, DNA metabolism, Humans, RNA Editing, Somatic Hypermutation, Immunoglobulin genetics, AICDA (Activation-Induced Cytidine Deaminase), Antibody Diversity, Cytidine Deaminase metabolism

Abstract

Activation-induced cytidine deaminase (AID) is an essential enzyme to regulate class switch recombination (CSR), somatic hypermutation (SHM), and gene conversion (GC). AID is known to be required for DNA cleavage of S regions in CSR. However, its molecular mechanism is a focus of extensive debate. RNA editing hypothesis postulates that AID edits yet unknown mRNA to generate specific endonucleases for CSR and SHM. By contrast, DNA deamination hypothesis assumes that AID deaminates cytosine in DNA, followed by DNA cleavage by base excision repair enzymes. We discuss available evidence for the two proposed models. Recent findings, namely requirement of protein synthesis for DNA breakage and dispensability of U removal activity of uracil DNA glycosylase, force us to reconsider DNA deamination hypothesis.

Published

2004

7. In vitro deamination of cytosine to uracil in single-stranded DNA by apolipoprotein B editing complex catalytic subunit 1 (APOBEC1).

Author

Petersen-Mahrt SK and Neuberger MS

Subjects

APOBEC-1 Deaminase, Animals, Base Sequence, Catalytic Domain, Chromatography, Ion Exchange, Cytidine Deaminase chemistry, Cytidine Deaminase isolation & purification, DNA Primers, DNA, Single-Stranded chemistry, Deamination, Rats, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Cytidine Deaminase metabolism, Cytosine metabolism, DNA, Single-Stranded metabolism, Uracil metabolism

Abstract

Apolipoprotein B-editing complex catalytic subunit 1 (APOBEC1) is the catalytic component of an RNA-editing complex that deaminates C6666 --> U in apolipoprotein B RNA in gastrointestinal tissue, thereby generating a premature stop codon. Whereas RNA is the physiological substrate of APOBEC1, recent experiments have strongly indicated that, when expressed in bacteria, APOBEC1 and some of its homologues can deaminate cytosine in DNA. Indeed, genetic evidence demonstrates that the physiological function of activation-induced deaminase, a B lymphocyte-specific APOBEC1 homologue, is to perform targeted deamination of cytosine within the immunoglobulin locus, thereby triggering antibody gene diversification. However, biochemical evidence of in vitro DNA deamination by members of the APOBEC family is still needed. Here, we show that deamination of cytosine to uracil in DNA can be achieved in vitro using partially purified APOBEC1 from extracts of transformed Escherichia coli. Thus, APOBEC1 can deaminate cytosine in both RNA and DNA. Strikingly, its activity on DNA is specific for single-stranded DNA and exhibits dependence on local sequence context.

Published

2003

8. Possible role of two phenylalanine residues in the active site of human cytidine deaminase.

Author

Vincenzetti S, Cambi A, Maury G, Bertorelle F, Gaubert G, Neuhard J, Natalini P, Salvatori D, De Sanctis G, and Vita A

Subjects

Binding Sites, Circular Dichroism, Cloning, Molecular, Cytidine Deaminase chemistry, Cytidine Deaminase genetics, Cytidine Deaminase isolation & purification, Enzyme Stability, Escherichia coli, Fluorescence, Humans, Kinetics, Mutagenesis, Site-Directed, Oxidation-Reduction, Pyrimidine Nucleosides metabolism, Tryptophan metabolism, Cytidine Deaminase metabolism, Phenylalanine metabolism

Abstract

Site-directed mutagenesis on human cytidine deaminase (CDA) was employed to mutate specifically two highly conserved phenylalanine residues, F36 and F137, to tryptophan; at the same time, the unique tryptophan residue present in the sequence at position 113 was mutated to phenylalanine. These double mutations were performed in order to have for each protein a single tryptophan signal for fluorescence studies relative to position 36 or 137. The mutant enzymes thus obtained, W113F, F36W/W113F and F137W/W113F, showed by circular dicroism and thermal stability an overall structure not greatly affected by the mutations. The titration of Trp residues by N-bromosuccinimide (NBS) suggested that residue W113 of the wild-type CDA and W36 of mutant F36W/W113F are buried in the tertiary structure of the enzyme, whereas the residue W137 of mutant F137W/W113F is located near the surface of the molecule. Kinetic experiments and equilibrium experiments with FZEB showed that the residue W113 seems not to be part of the active site of the enzyme whereas the Phe/Trp substitution in F36W/W113F and F137W/W113F mutant enzymes had a negative effect on substrate binding and catalysis, suggesting that F137 and F36 of the wild-type CDA are involved in a stabilizing interaction between ligand and enzyme.

Published

2000

9. Human apolipoprotein B RNA editing deaminase gene (APOBEC1).

Author

Fujino T, Navaratnam N, and Scott J

Subjects

APOBEC-1 Deaminase, Alternative Splicing, Amino Acid Sequence, Animals, Apolipoproteins B metabolism, Base Sequence, Caco-2 Cells, Cloning, Molecular, Cytidine Deaminase chemistry, Cytidine Deaminase isolation & purification, Humans, Mice, Molecular Sequence Data, RNA Processing, Post-Transcriptional, Rabbits, Rats, Transcription, Genetic, AICDA (Activation-Induced Cytidine Deaminase), Cytidine Deaminase genetics, RNA Editing genetics

Abstract

Genomic clones encoding the human APOBEC1 gene and its 5' flanking region have been isolated and characterized. The human gene contains five coding exons. The introns dividing these exons correspond exactly to those found in the mouse gene. The translation initiation site, ATG, is located in exon 2 at the same site as in the mouse. The 5' flanking sequence contains two Alu repeats of the Sq family. Primer extension analysis demonstrated the presence of two major transcription initiation sites. The first transcription initiation site delineates the beginning of a noncoding first exon and resides downstream of the first Alu sequence. The second transcription initiation site is within the second Alu repeat. This Alu repeat resides within the first intron, which is spliced out of the transcript from the first start site. Neither transcription initiation site has a TATA or CCAT box. Comparison with the mouse gene suggests that the Alu sequence insertion split the intestinal promoter and that subsequently the down-stream Alu sequence took on a promoter function. No evidence was found for a far upstream non-tissue-specific promoter similar to that demonstrated in the mouse gene. Rather, consideration of results from the marsupial APOBEC-1 gene suggests that this upstream mouse promoter may have had a later evolutionary origin.

Published

1998

10. Developmental regulation of the catalytic subunit of the apolipoprotein B mRNA editing enzyme (APOBEC-1) in human small intestine.

Author

Giannoni F, Chou SC, Skarosi SF, Verp MS, Field FJ, Coleman RA, and Davidson NO

Subjects

APOBEC-1 Deaminase, Acyltransferases metabolism, Adult, Apolipoproteins B, Base Sequence, Cells, Cultured, Child, Coenzyme A Ligases metabolism, Cytidine Deaminase genetics, Cytidine Deaminase isolation & purification, Diacylglycerol O-Acyltransferase, Fetus, Humans, Immunohistochemistry, Intestine, Small enzymology, Liver enzymology, Molecular Sequence Data, Polymerase Chain Reaction, RNA, Messenger analysis, Long-Chain-Fatty-Acid-CoA Ligase, AICDA (Activation-Induced Cytidine Deaminase), Cytidine Deaminase biosynthesis, Gene Expression Regulation, Developmental, Intestine, Small growth & development, Repressor Proteins, Saccharomyces cerevisiae Proteins

Abstract

Apolipoprotein (apo) B mRNA editing is a site-specific cytidine deamination reaction responsible for the production of apoB-48 in mammalian small intestine. This process is mediated by an enzyme complex that includes the catalytic subunit, APOBEC-1. In the present study, it is shown that the developmental regulation of apoB mRNA editing in fetal human small intestine is closely mirrored by accumulation of APOBEC-1 mRNA. Similar results were obtained using Caco-2 cells, the data further suggesting that culture of these cells under conditions previously shown to promote differentiation produce an earlier and more marked induction of APOBEC-1 mRNA abundance. Complementary analysis of APOBEC-1 protein accumulation using immunocytochemical localization reveals its appearance to be temporally coordinated with the accumulation of APOBEC-1 mRNA and its distribution to be confined to villus-associated enterocytes. Previous studies demonstrated a close temporal association between the development of triglyceride synthesis and apoB mRNA editing in the rat liver and small intestine. Analysis of fatty acid CoA ligase, monoacylglycerol acyltransferase, and diacylglycerol acyltransferase activity in preparations of human liver and small intestine demonstrates activity of all three enzymes in the late first and early second trimester, suggesting that certain aspects of complex lipid biosynthesis in the human fetal small intestine and liver are regulated developmentally. The cues that modulate the post-transcriptional regulation of fetal human small intestinal apoB gene expression may thus include both temporal programming and events related to the emergence of lipid transport capability.

Published

1995

11. Human cytidine deaminase: purification of enzyme, cloning, and expression of its complementary DNA.

Author

Laliberté J and Momparler RL

Subjects

Amino Acid Sequence, Base Sequence, Cell Line, Chromosomes, Human, Pair 1, Cytidine Deaminase chemistry, Cytidine Deaminase isolation & purification, DNA, Complementary genetics, Escherichia coli enzymology, Humans, Molecular Sequence Data, Molecular Weight, Placenta enzymology, Cytidine Deaminase genetics

Abstract

Cytidine (CR) deaminase was purified 47,000-fold to homogeneity from human placenta. The molecular mass of CR deaminase was estimated to be 48.7 kDa by gel filtration and 16.1 kDa by sodium dodecyl sulfate polyacrylamide gel electrophoresis, suggesting that it contains three or four identical subunits. We determined the amino acid sequence of several peptide fragments and designed 5'-primers to amplify, by the polymerase chain reaction, a specific 364-base pair DNA fragment using human liver complementary DNA (cDNA) as the template. This DNA fragment, which contains the codons of one peptide, was used as a probe to screen a cDNA library from human liver. We isolated and sequenced a cDNA clone of 910 base pairs that contained a 5' nontranslated region, a 438-base pair coding region, and a 3' nontranslated region with a polyadenylated tail. The translated region of the clone contained a deduced sequence of 146 amino acids, with a predicted molecular mass of 16.2 kDa and the sequences of our peptides. The cDNA was ligated in pGEX vector and expressed in Escherichia coli. The expressed protein had a high CR deaminase activity and molecular mass of 16.3 kDa. These data demonstrate clearly that the open reading frame of our cDNA clone codes for a functional human CR deaminase. Polymerase chain reaction amplifications of gene-specific DNA fragments from human/rodent hybrid cells indicate the localization of CR deaminase gene to human chromosome 1. The cDNA for CR deaminase will be a useful molecular probe to investigate the importance of this enzyme in chemotherapy.

Published

1994

12. Purification and properties of cytidine deaminase from escherichia coli.

Author

Ashley GW and Bartlett PA

Subjects

Borates pharmacology, Chromatography, Affinity methods, Cytidine Deaminase metabolism, Kinetics, Molecular Weight, Substrate Specificity, Cytidine Deaminase isolation & purification, Escherichia coli enzymology, Nucleoside Deaminases isolation & purification

Abstract

A convenient and efficient procedure for the purification of cytidine deaminase (EC 3.5.4.5) from Escherichia coli is reported. The key step involves adsorption of the enzyme from a crude ammonium sulfate fraction onto a cytidine-containing affinity resin, followed by elution with 0.5 M borate buffer. Subsequent chromatography on DEAE-Sepharose results in an overall 1690-fold purification, yielding enzyme with a specific activity of 118 units/mg. Cytidine deaminase has an apparent molecular weight of 54,000 as determined by gel filtration, whereas sodium dodecyl sulfate-polyacrylamide gel electrophoresis shows a band at molecular weight 35,000. Cytidine deaminase is inhibited by 5-(chloromercuri)cytidine with kinetic behavior typical of active-site-directed inactivation, with KD = 0.09 mM and kinact = 1.25 min-1. The enzyme is protected against inactivation in the presence of substrate, and the inhibition is reversed with high concentrations of mercaptoethanol. This suggests that inactivation is the result of a mercaptide formation between the mercury and an active-site thiol.

Published

1984