Reduction of the P5A-ATPase Spf1p phosphoenzyme by a Ca2+-dependent phosphatase

Corradi, Gerardo R.; Mazzitelli, Luciana R.; Petrovich, Guido Daniel; Grenón, Paula; Sørensen, Danny Mollerup; Palmgren, Michael G.; Pinto, Felicitas de Tezanos; Adamo, Hugo P.

doi:10.1371/journal.pone.0232476

Cited by 8 publications

(6 citation statements)

References 44 publications

(68 reference statements)

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“…Total membranes from eight liters of yeasts expressing the recombinant protein were obtained as previously described [ 24 , 44 ]. Briefly, the microsomal membranes were solubilized at 4°C for 30 min by adding 2 g of Triton X-100/g of total membrane proteins and the supernatant was loaded onto a column with 2-ml nickel-nitrilotriacetic acid—agarose resin (Qiagen).…”

Section: Methodsmentioning

confidence: 99%

“…Briefly, the microsomal membranes were solubilized at 4°C for 30 min by adding 2 g of Triton X-100/g of total membrane proteins and the supernatant was loaded onto a column with 2-ml nickel-nitrilotriacetic acid—agarose resin (Qiagen). The purification was carried out following the protocol for the production of “pure Spf1p” previously described [ 44 ]. Finally, the protein was eluted in purification buffer containing 0.005% C 12 E 10 and 150 mM imidazole.…”

Section: Methodsmentioning

confidence: 99%

“…The ATPase activity was estimated at 28°C by measuring the release of Pi from ATP using the colorimetric method of Baginski [ 45 ] as previously described [ 44 ]. Reaction medium was identical to that used for proteolysis and contained 1 μg of Spf1p supplemented with PC plus 3 mM ATP.…”

Section: Methodsmentioning

confidence: 99%

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Highly exposed segment of the Spf1p P5A-ATPase near transmembrane M5 detected by limited proteolysis

et al. 2021

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The yeast Spf1p protein is a primary transporter that belongs to group 5 of the large family of P-ATPases. Loss of Spf1p function produces ER stress with alterations of metal ion and sterol homeostasis and protein folding, glycosylation and membrane insertion. The amino acid sequence of Spf1p shows the characteristic P-ATPase domains A, N, and P and the transmembrane segments M1-M10. In addition, Spf1p exhibits unique structures at its N-terminus (N-T region), including two putative additional transmembrane domains, and a large insertion connecting the P domain with transmembrane segment M5 (D region). Here we used limited proteolysis to examine the structure of Spf1p. A short exposure of Spf1p to trypsin or proteinase K resulted in the cleavage at the N and C terminal regions of the protein and abrogated the formation of the catalytic phosphoenzyme and the ATPase activity. In contrast, limited proteolysis of Spf1p with chymotrypsin generated a large N-terminal fragment containing most of the M4-M5 cytosolic loop, and a minor fragment containing the C-terminal region. If lipids were present during chymotryptic proteolysis, phosphoenzyme formation and ATPase activity were preserved. ATP slowed Spf1p proteolysis without detectable changes of the generated fragments. The analysis of the proteolytic peptides by mass spectrometry and Edman degradation indicated that the preferential chymotryptic site was localized near the cytosolic end of M5. The susceptibility to proteolysis suggests an unexpected exposure of this region of Spf1p that may be an intrinsic feature of P5A-ATPases.

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Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

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Highly exposed segment of the Spf1p P5A-ATPase near transmembrane M5 detected by limited proteolysis

et al. 2021

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“…Spf1p was expressed and purified using a protocol that was previously optimized to remove contaminants that can interfere with Spf1p activity [ 12 , 23 ]. The purified preparations were confirmed to contain mainly Spf1p protein as determined by amino acid analysis and mass spectrometry, although in some of the produced fractions we could identify glyderaldehyde-3-phosphate dehydrogenase as a minor contaminant ( S1 Fig ).…”

Section: Resultsmentioning

confidence: 99%

Section: Ethylene-glycol Containing Detergents Increase Atpase Activi...mentioning

confidence: 99%

ATP hydrolytic activity of purified Spf1p correlate with micellar lipid fluidity and is dependent on conserved residues in transmembrane helix M1

Ipsen

Sørensen²

2022

PLoS ONE

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P5A ATPases are expressed in the endoplasmic reticulum (ER) of all eukaryotic cells, and their disruption results in pleiotropic phenotypes related to severe ER stress. They were recently proposed to function in peptide translocation although their specificity have yet to be confirmed in reconstituted assays using the purified enzyme. A general theme for P-type ATPases is that binding and transport of substrates is coupled to hydrolysis of ATP in a conserved allosteric mechanism, however several independent reports have shown purified Spf1p to display intrinsic spontaneous ATP hydrolytic activity after purification. It has never been determined to what extend this spontaneous activity is caused by uncoupling of the enzyme. In this work we have purified a functional tagged version of the Saccharomyces cerevisiae P5A ATPase Spf1p and have observed that the intrinsic ATP hydrolytic activity of the purified and re-lipidated protein can be stimulated by specific detergents (C12E8, C12E10 and Tween20) in mixed lipid/detergent micelles in the absence of any apparent substrate. We further show that this increase in activity correlate with the reaction temperature and the anisotropic state of the mixed lipid/detergent micelles and further that this correlation relies on three highly conserved phenylalanine residues in M1. This suggests that at least part of the intrinsic ATP hydrolytic activity is allosterically coupled to movements in the TM domain in the purified preparations. It is suggested that free movement of the M1 helix represent an energetic constraint on catalysis and that this constraint likely is lost in the purified preparations resulting in protein with intrinsic spontaneous ATP hydrolytic activity. Removal of the N-terminal part of the protein apparently removes this activity.

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The effect of metal ions on the Spf1p P5A-ATPase. High sensitivity to irreversible inhibition by zinc

Petrovich¹,

Corradi²,

Adamo³

2022

Archives of Biochemistry and Biophysics

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Reduction of the P5A-ATPase Spf1p phosphoenzyme by a Ca2+-dependent phosphatase

Cited by 8 publications

References 44 publications

Highly exposed segment of the Spf1p P5A-ATPase near transmembrane M5 detected by limited proteolysis

Highly exposed segment of the Spf1p P5A-ATPase near transmembrane M5 detected by limited proteolysis

ATP hydrolytic activity of purified Spf1p correlate with micellar lipid fluidity and is dependent on conserved residues in transmembrane helix M1

The effect of metal ions on the Spf1p P5A-ATPase. High sensitivity to irreversible inhibition by zinc

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