Mutational Analysis of the Catalytic Subunit of the Yeast Vacuolar Proton-Translocating ATPase

Liu, Jianzhong; Kane, Patricia M.

doi:10.1021/bi9608065

Cited by 56 publications

(69 citation statements)

References 57 publications

(108 reference statements)

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“…The plasmid pPK17-7, containing VMA1 lacking the entire VMA1-derived endonuclease (VDE) subcloned into the yeast shuttle vector pSEYC68 at BamHI and SalI sites (24,35) was from Dr. Kane. Yeast cells were grown in yeast extract-peptone-dextrose (YEPD) medium or in supplemented synthetic dextrose medium (SD).…”

Section: Materials and Strains-zymolyasementioning

confidence: 99%

“…Deletion of genes encoding subunits of the V-ATPase results in a conditional lethal phenotype (35,47,48), which is also observed for vma mutants possessing less than approximately 20% of wild-type V-ATPase activity (24). Strains bearing these mutations are able to grow on medium buffered to acidic pH (5.0 -5.5) but are unable to grow at neutral pH (7.5) or in neutral medium containing 50 mM CaCl 2 .…”

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confidence: 92%

“…The F-ATPases function in ATP synthesis in mitochondria, chloroplasts, and bacteria (18 -20). The x-ray crystal structures of F 1 indicate that the nucleotide binding sites are located at the interface of the ␤ and ␣ subunits, with the catalytic sites residing primarily on the ␤ subunits and the noncatalytic sites residing primarily on the ␣ subunits (21,22).Although mutagenesis studies of the yeast V-ATPase have begun to identify residues important for catalytic activity (23)(24)(25)(26), the structure of the nucleotide binding sites on the VATPase has yet to be determined. One approach to characterizing the structure of nucleotide binding sites is the use of photoaffinity analogs.…”

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confidence: 99%

“…Although mutagenesis studies of the yeast V-ATPase have begun to identify residues important for catalytic activity (23)(24)(25)(26), the structure of the nucleotide binding sites on the VATPase has yet to be determined. One approach to characterizing the structure of nucleotide binding sites is the use of photoaffinity analogs.…”

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Photoaffinity Labeling of Wild-type and Mutant Forms of the Yeast V-ATPase A Subunit by 2-Azido-[32P]ADP

MacLeod¹,

Vasilyeva²,

Merdek³

et al. 1999

Journal of Biological Chemistry

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To test the proximity of these aromatic residues to the adenine ring, the yeast V-ATPase containing wild-type and mutant forms of the A subunit was reacted with 2-azido-[ 32 P]ADP, a photoaffinity analog that stably modifies tyrosine but not phenylalanine residues. Mutant forms of the A subunit were constructed in which the two endogenous tyrosine residues were replaced with phenylalanine and in which a single tyrosine was introduced at each of the four positions. Strong ATP-protectable labeling of the A subunit was observed for the wild-type and the mutant containing tyrosine at 532, significant ATP-protectable labeling was observed for the mutants containing tyrosine at positions 452 and 538, and only very weak labeling was observed for the mutants containing tyrosine at 535 or in which all four residues were phenylalanine. These results suggest that Tyr 532 and possibly Phe 452 and Tyr 538 are in close proximity to the adenine ring of ATP bound to the A subunit. In addition, the effects of mutations at Phe 452 , Tyr 532 , Tyr 535 , and Glu 286 on dissociation of the peripheral V 1 and integral V 0 domains both in vivo and in vitro were examined. The results suggest that in vivo dissociation requires catalytic activity while in vitro dissociation requires nucleotide binding to the catalytic site.The vacuolar proton-translocating ATPases (or V-ATPases) 1 are a family of ATP-dependent proton pumps responsible for acidification of intracellular compartments in eukaryotic cells (1-6). The V-ATPases function in a variety of cellular processes, including protein processing and degradation, receptormediated endocytosis, intracellular membrane traffic, and coupled transport (1-6). For certain specialized cells, including renal intercalated cells (7), macrophages and neutrophils (8), tumor cells (9), and osteoclasts (10), the V-ATPase has been identified at the plasma membrane and acidifies the extracellular space. In yeast, acidification of the central vacuole by the V-ATPase serves to activate protein degradation and to drive the uptake of solutes such as Ca 2ϩ and amino acids for storage (5).The V-ATPases are composed of two domains, a peripheral, cytoplasmic 570-kDa V 1 domain responsible for nucleotide binding and hydrolysis, and a membrane integral 260-kDa V 0 domain responsible for proton translocation across the membrane (1-6). The V 1 domain contains eight different subunits (subunits A-H, with molecular masses 70 -14 kDa) while the V 0 domain contains five different subunits (subunits a, d, cЉ, c, and cЈ, with molecular masses from 100 to 17 kDa). The nucleotide binding subunits have been identified as the A and B subunits, which are believed to form a hexameric structure containing three copies of each subunit (11).Previous studies have demonstrated that the catalytic sites reside on the A subunits and that a second class of sites, termed "noncatalytic" sites, reside on the B subunits, giving a total of six nucleotide binding sites per complex (12-15). The A and B subunits of the V-ATPase are approximately 2...

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Section: Materials and Strains-zymolyasementioning

confidence: 99%

mentioning

confidence: 92%

mentioning

confidence: 99%

mentioning

confidence: 99%

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Photoaffinity Labeling of Wild-type and Mutant Forms of the Yeast V-ATPase A Subunit by 2-Azido-[32P]ADP

MacLeod¹,

Vasilyeva²,

Merdek³

et al. 1999

Journal of Biological Chemistry

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“…All mutant strains were tested for growth on YEPD buffered to pH 5.5 or 7.5. Yeast that contain Ͻ20% wild-type V-ATPase activity are unable to grow at neutral pH (35). This conditional lethality is referred to as the vma Ϫ phenotype (36).…”

Section: Construction Of Single Cysteine-containing Mutants Of Vph1p mentioning

confidence: 99%

Structural Analysis of the N-terminal Domain of Subunit a of the Yeast Vacuolar ATPase (V-ATPase) Using Accessibility of Single Cysteine Substitutions to Chemical Modification

Liberman

Cotter

Baleja

et al. 2013

Journal of Biological Chemistry

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Background:The N terminus of the V-ATPase subunit a functions in intracellular targeting and regulation of assembly.Results: A homology model of this domain was tested by determining aqueous accessibility of introduced cysteines. Conclusion:The results identify residues located at the peripheral/integral domain interface. Significance: The identified sites may participate in interactions that regulate V-ATPase assembly.

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Isolation of the V-ATPase A and c subunit cDNAs from mosquito midgut and malpighian tubules

Gill

Chu

Smethurst

et al. 1998

Arch. Insect Biochem. Physiol.

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Using conserved amino acid sequences for the design of oligonucleotide primers, we isolated cDNA clones for two subunits of the V‐ATPase from the midgut and Malpighian tubules of Aedes aegypti larvae. The 3.1 kb cDNA of the A subunit of the peripheral catalytic V1 sector codes for a protein of 68.6 kDa. The protein contains conserved motifs, including an ATP/GTP binding site, found in all other A subunits. Southern analysis using the A subunit as a probe suggests the presence of only a single copy of gene in the Aedes aegypti. The 0.85 kb cDNA of the c subunit of the membrane H+ conducting V0 sector codes for a protein of kDa. This protein has four transmembrane domains and contains a conserved glutamic acid that serves as the binding site for dicyclohexylcarbodiimide. Southern analysis using the c subunit as a probe suggests the presence of more than one related gene in the genome of Aedes aegypti. Pileup analysis of various A and c subunits shows that these subunits fall into distinct clusters, including one in which all arthropod proteins are clustered. Arch. Insect Biochem. Physiol. 37:80–90, 1998. © 1998 Wiley‐Liss, Inc.

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Mutational Analysis of the Catalytic Subunit of the Yeast Vacuolar Proton-Translocating ATPase

Cited by 56 publications

References 57 publications

Photoaffinity Labeling of Wild-type and Mutant Forms of the Yeast V-ATPase A Subunit by 2-Azido-[32P]ADP

Photoaffinity Labeling of Wild-type and Mutant Forms of the Yeast V-ATPase A Subunit by 2-Azido-[32P]ADP

Structural Analysis of the N-terminal Domain of Subunit a of the Yeast Vacuolar ATPase (V-ATPase) Using Accessibility of Single Cysteine Substitutions to Chemical Modification

Isolation of the V-ATPase A and c subunit cDNAs from mosquito midgut and malpighian tubules

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