Purification and general properties of the DNA-binding protein (P16) from rat liver mitochondria.

Pavco, Pamela A.; Tuyle, G C Van

doi:10.1083/jcb.100.1.258

Cited by 42 publications

(20 citation statements)

References 20 publications

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“…E. coli SSB is known to bind DNA in several modes depending on ionic conditions (29). Studies of mtSSBs also show salt-dependent effects on DNA binding and, in particular, upon binding-site size and cooperativity of DNA binding (5,11,18). Ionic conditions likely affect both DNA conformation and SSB structure and, hence, its interactions with pol ␥.…”

Section: Discussionmentioning

confidence: 99%

Physiological and Biochemical Defects in Functional Interactions of Mitochondrial DNA Polymerase and DNA-binding Mutants of Single-stranded DNA-binding Protein

Farr

Matsushima

Lagina

et al. 2004

Journal of Biological Chemistry

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Mitochondrial biogenesis is a key process in animal cell proliferation, and mtDNA replication is an essential component of that process. Whereas a large number of proteins participate in multi-component replication machines in bacterial and nuclear systems, a minimal set of essential proteins are likely involved in the mtDNA replication process (1). We have demonstrated functional interactions between the two-subunit Drosophila mitochondrial DNA polymerase (pol ␥) 1 and the homotetrameric mitochondrial single-stranded DNA-binding protein, mtSSB, at the levels of template-primer binding and initiation and elongation of DNA strand synthesis (2). These studies have documented roles for mtSSB in enhancing primer recognition and binding and in stimulation by 20-to 30-fold of the rate of initiation of DNA strands by pol ␥. Moreover, mtSSB increases severalfold the processivity of pol ␥ in DNA strand elongation.To probe further the biochemical and physiological importance of these functional interactions, we have evaluated the effects of altered forms of mtSSB on DNA binding per se and upon the coordinated reactions involving mtSSB and pol ␥. We find that even modest DNA-binding defects in mtSSB substantially affect DNA synthesis by pol ␥. Furthermore, under conditions that reduce cellular levels of endogenous wild-type mtSSB, a mtDNA depletion phenotype develops that is rescued by production of exogenous wild-type but not mutant mtSSB. EXPERIMENTAL PROCEDURESNucleotides and Nucleic Acids-Unlabeled deoxy-and ribonucleotides were purchased from Amersham Biosciences. [ 3 H]dTTP, [␣-32 P]dATP, and [␥-32 P]ATP were purchased from ICN Biochemicals. Wild-type (6,407 nucleotides (nt)) and recombinant (10,650 nt) M13 DNAs were prepared by standard laboratory methods. Oligodeoxynucleotides complementary to the M13 viral DNAs were synthesized in an Applied Biosystems oligonucleotide synthesizer. The primer for the recombinant M13 DNA that was used in the pol ␥ stimulation assay was 17 nt in length and the primer for the M13 wild-type DNA used in the processivity analysis was 15 nt in length. To prepare template primers for DNA synthesis, M13 DNAs were added to the 15-and 17-mer oligonucleotide primers to a concentration of ϳ70 mM (as nt, in 4-fold molar excess over homologous oligonucleotide), and the DNA mixtures were precipitated with ethanol. The pellets were resuspended in a buffer (0.1 ml) containing 10 mM Tris-HCl, pH 8.0, 0.3 M NaCl, and 0.03 M sodium citrate and were incubated at 65°C for 1 h, followed by incubation at 37°C for an additional hour to anneal the primer to the template. The sequence of the 38-mer oligonucleotide used in the DNA binding and gel mobility shift assays (GMSA) is complementary to positions 6291-6329 in M13mp7 DNA.Enzymes and Proteins-Drosophila DNA polymerase ␥ (Fraction VI, Ͼ90% homogeneous) was prepared from embryonic mitochondria, as described by Wernette and Kaguni (3). Recombinant Drosophila mtSSB (Ͼ90% homogeneous) was prepared as described by Farr et al. (2). T4 polynucleotide kinase and ...

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Section: Discussionmentioning

confidence: 99%

Physiological and Biochemical Defects in Functional Interactions of Mitochondrial DNA Polymerase and DNA-binding Mutants of Single-stranded DNA-binding Protein

Farr

Matsushima

Lagina

et al. 2004

Journal of Biological Chemistry

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“…They suggest that, although there is variation in the central portion of TAS among different species, all begin with the sequence ACAT at their 5' end, are quite A+T rich, and end with a 3' A-T sequence. It is possible that differences in the nuclear-encoded gene products which may be involved in mtDNA sequence recognition (1,20,23) …”

Section: Discussionmentioning

confidence: 99%

Template-directed arrest of mammalian mitochondrial DNA synthesis.

MacKay¹,

Olivo²,

Laipis³

et al. 1986

Mol. Cell. Biol.

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Mammalian mitochondrial DNA often contains a short DNA displacement loop at the heavy-strand origin of replication. This short nascent DNA molecule has been used to study site-specific termination of mitochondrial DNA synthesis in human and mouse cells. We examined D-loop strand termination in two distantly related artiodactyls, the pig and the cow. Porcine mitochondrial DNA was unique among mammals in that it contained only a single species of D-loop single-stranded DNA. Its 3' end mapped to a site 187 nucleotides from the 5' end of the proline tRNA gene. This site was 21 and 47 nucleotides 5' to two very similar sequences (5' ACATATPyATTAT 3') which are closely related to the human and mouse termination-associated sequences noted by Doda et al. (J. N. Doda, D. T. Wright, and D. A. Clayton, Proc. Nat. Acad. Sci. USA 78:616-6120, 1981). Bovine mitochondrial DNA contained three major D-loop DNA species whose 3' ends mapped to three different sites. These sites were not found in the porcine sequence. However, the bovine termination sites were located 60 to 64 base pairs 5' from sequences which were also very similar to the termination-associated sequences present in pigs and other mammals. These results firmly establish the concept that arrest of heavy-strand DNA synthesis is an event determined, at least in part, by template sequence. They also suggest that arrest is determined by sequences which are a considerable physical distance away from the actual termination site.Mitochondrial DNA (mtDNA) in mammalian cells exists as a covalently closed, circular, supercoiled, doublestranded DNA molecule approximately 16,000 base pairs in length (13). Each strand is replicated unidirectionally from a separate origin. Although synthesis of daughter heavy (H) strands begins at discrete genome locations, the precise nucleotide sequence requirements for H-strand initiation have not yet been determined and appear to vary considerably among mammals (10). After initiation, most newly initiated H strands terminate <700 nucleotides downstream. This leads to a partial relaxation of parental supercoiled molecules because the short, newly synthesized H strand, variously termed D-loop strand (11), 12,15,19), or DH-DNA (7-9), remains associated with the template, thus creating a triple-stranded structure known as a displacement loop (D-loop) molecule. The major form of mammalian mtDNA isolated from cells is this triplestranded, partially replicated D-loop molecule (10).Previous studies mapping the 3' ends of D-loop strands suggested that a portion of the template sequence may be involved in the arrest of H-strand synthesis within the D-loop region. D-loop molecules isolated from mouse L cells contain four major D-loop strands with four distinct 3' ends (11), while those of human HeLa cells contain three major D-loop strands but only one major 3' end (12). The existence of a conserved nucleotide sequence approximately 30 to 60 nucleotides from each 3' end prompted Doda et al. (11) to propose that this sequence may play a role in determ...

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“…In higher organisms mtSSB is primarily detected in mitochondria. Trace amounts have, however, been detected in the nucleus (77,78), and it has been demonstrated that overexpression of mtSSB can result in the activation of a nuclear gene, A␣ fibrinogen (78). Interestingly, a nuclear protein with N-terminal sequence conserved with mature mtSSB was isolated as binding to an IL-6 response element in the A␣ fibrinogen gene (78).…”

Section: An Ordered Arrangement Of Repressor Elements Binding Csd Promentioning

confidence: 99%

An Ordered Array of Cold Shock Domain Repressor Elements across Tumor Necrosis Factor-responsive Elements of the Granulocyte-Macrophage Colony-stimulating Factor Promoter

Coles¹,

Diamond²,

Occhiodoro³

et al. 2000

Journal of Biological Chemistry

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The tumor necrosis factor-␣-responsive region of the human granulocyte-macrophage colony-stimulating factor (GM-CSF) promoter (؊114 to ؊31) encompasses binding sites for NF-B, CBF, AP-1, ETS, and NFAT families of transcription factors. We show both here and previously that mutation of any one of these binding sites greatly reduces tumor necrosis factor-␣ induction of the GM-CSF promoter. Interspersed between these elements are sequences that when mutated lead to an increase in GM-CSF promoter activity. We have previously shown that two of these repressor elements bind proteins known as cold shock domain (CSD) factors and that overexpression of CSD proteins leads to repression of GM-CSF promoter activity in fibroblasts. CSD proteins are single strand DNA-and RNA-binding proteins that contact 5-CCTG-3 sequences in the GM-CSF repressor elements. We show here that two newly identified repressor sequences in the proximal promoter can also bind CSD proteins. We have characterized the CSDcontaining protein complexes that bind to the GM-CSF promoter and identified a novel protein related to mitochondrial single strand binding protein that forms part of one of these complexes. The four CSD-binding sites on the promoter occur in pairs on opposite strands of the DNA and appear to form an ordered array of binding elements. A similar ordered array of CSD sites are present in the promoters of the granulocyte colony-stimulating factor and interleukin-3 genes, implying a common mechanism for negative regulation of these myeloid growth factors.

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Purification and general properties of the DNA-binding protein (P16) from rat liver mitochondria.

Cited by 42 publications

References 20 publications

Physiological and Biochemical Defects in Functional Interactions of Mitochondrial DNA Polymerase and DNA-binding Mutants of Single-stranded DNA-binding Protein

Physiological and Biochemical Defects in Functional Interactions of Mitochondrial DNA Polymerase and DNA-binding Mutants of Single-stranded DNA-binding Protein

Template-directed arrest of mammalian mitochondrial DNA synthesis.

An Ordered Array of Cold Shock Domain Repressor Elements across Tumor Necrosis Factor-responsive Elements of the Granulocyte-Macrophage Colony-stimulating Factor Promoter

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