Characterization of the ATPase Activity of Purified Chinese Hamster P-glycoprotein

Urbatsch, Ina L.; Al‐Shawi, Marwan K.; Senior, Alan E.

doi:10.1021/bi00189a008

Cited by 217 publications

(229 citation statements)

References 37 publications

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“…4), PgP had been purified using conditions optimized for its own recovery, and the preparation showed a basal ATPase activity and response to substrate consistent with what one expects for the fully functioning molecule (Table I). As a consequence, we conclude that nucleotide binding by CFTR is comparable to that shown by Pgp [36,38]. We also note that CFTR catalyzes a net hydrolysis of ATP (Fig.…”

Section: Purification Of Functional Cftrsupporting

confidence: 64%

“…Indeed, when the data were expressed on a molar basis (with correction for protein content and molecular weight), we concluded that CFTR and Pgp bind nucleotide (Az-ATP) with approximately equal efficiency (109% vs. 100%, respectively). Since the biochemical characteristics of Pgp purified from Sf9 cells (e.g., V max , K M , and substrate stimulation) match values cited in the literature for the fully functioning molecule [33,[35][36][37][38] (Table I), we conclude that nucleotide processing by purified CFTR exhibits characteristics similar to that of Pgp.In mammalian systems, R domain phosphorylation must occur before CFTR chloride channel function is observed. However, in Sf9 cells, the CFTR-mediated anion conductance appears without addition of exogenous stimuli that might activate intracellular protein kinases and promote R domain phosphorylation [13].…”

supporting

confidence: 71%

“…We also evaluated recovery of functional CFTR in a quantitative manner by comparing nucleotide trapping of CFTR in parallel with that of its well-characterized relative, Pgp, which had been expressed in Sf9 cells and purified and reconstituted using conditions optimized for its own recovery [33,[35][36][37]38] (Table I, Fig. 4c-e).…”

Section: Nucleotide Processing By Purified and Reconstituted Cftrmentioning

confidence: 99%

“…4ab). This behavior, noted by others in studies of crude membranes [14,15], has not been reported for other ABC transporters [14,15,33] and may be a distinctive feature of CFTR.We also evaluated recovery of functional CFTR in a quantitative manner by comparing nucleotide trapping of CFTR in parallel with that of its well-characterized relative, Pgp, which had been expressed in Sf9 cells and purified and reconstituted using conditions optimized for its own recovery [33,[35][36][37]38] (Table I, Fig. 4c-e).…”

mentioning

confidence: 96%

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Characterization of the Adenosinetriphosphatase and Transport Activities of Purified Cystic Fibrosis Transmembrane Conductance Regulator

2004

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The cystic fibrosis transmembrane conductance regulator (CFTR) functions in vivo as a cAMPactivated chloride channel. A member of the ATP-binding cassette superfamily of membrane transporters, CFTR contains two transmembrane domains (TMDs), two nucleotide-binding domains (NBDs), and a regulatory (R) domain. It is presumed that CFTR couples ATP hydrolysis to channel gating, and as a first step in addressing this issue directly, we have established conditions for purification of biochemical quantities of human CFTR expressed in Sf9 insect cells. Use of an 8-azido-[α 32 P]-ATP binding and vanadate-trapping assay allowed us to devise conditions to preserve CFTR function during purification of a C-terminal His 10 -tagged variant after solubilization with lyso-phosphatidylglycerol (1%) and diheptanolylphosphatidylcholine (0.3%) in the presence of excess phospholipid. Study of purified and reconstituted CFTR showed that it binds nucleotide with an efficiency comparable to that of P-glycoprotein, and that it hydrolyzes ATP at rates sufficient to account for presumed in vivo activity (V Max of 58 ± 5 nmol/min/mg protein, K M (MgATP) of 0.15 mM). In further work, we found that neither nucleotide binding nor ATPase activity were altered by phosphorylation (using Protein Kinase A) or dephosphorylation (with Protein Phosphatase 2B); we also observed inhibition (∼40%) of ATP hydrolysis by reduced glutathione, but not by DTT. To evaluate CFTR function as an anion channel, we introduced an in vitro macroscopic assay based on the equilibrium exchange of proteoliposome-entrapped radioactive tracers. This revealed a CFTRdependent transport of 125 I that could be inhibited by known chloride channel blockers; no significant CFTR-dependent transport of [α 32 P]-ATP was observed. We conclude that heterologous expression of CFTR in Sf9 cells can support manufacture and purification of fully functional CFTR. This should aid in further biochemical characterization of this important molecule.The Cystic Fibrosis Transmembrane conductance Regulator (CFTR) is the cAMP-activated chloride channel encoded by the gene defective in patients with the disease [1,2]. As a member of the ATP-Binding Cassette (ABC) superfamily of membrane transporters, CFTR shares a conserved architecture consisting of two homologous halves, each containing a transmembrane domain (TMD) and a nucleotide-binding domain (NBD). In CFTR, unlike other ABC transporters, a third domain, termed the regulatory (R) domain, is located between the two half molecules. Current evidence suggests that the TMDs define the CFTR chloride channel, while the NBDs and the R domain mediate channel gating [3][4][5][6][7][8][9][10][11] Although CFTR is glycosylated, there is currently no evidence indicating that the presence of carbohydrate affects CFTR structure or function [12]. Consistent with this presumption, expression of human CFTR in Sf9 insect cells results in appearance of the 140 kD core polypeptide -containing little or no glycosylation -that mediates a newly acquired anion ...

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Section: Purification Of Functional Cftrsupporting

confidence: 64%

supporting

confidence: 71%

Section: Nucleotide Processing By Purified and Reconstituted Cftrmentioning

confidence: 99%

mentioning

confidence: 96%

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Characterization of the Adenosinetriphosphatase and Transport Activities of Purified Cystic Fibrosis Transmembrane Conductance Regulator

2004

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“…Both halves of P-gp can hydrolyze ATP (14,15), but drug-stimulated ATPase activity (14) and conferring of drug resistance (16) requires interaction between the two halves of P-gp. Both halves of P-gp are required for activity because drug binding requires interaction between the NH 2 and COOHterminal TM domains (16) whereas both ATP binding sites are needed for ATPase activity (17)(18)(19)(20)(21) and the nucleotide-binding sites appear to function in an alternating mechanism (22).…”

mentioning

confidence: 99%

Vanadate trapping of nucleotide at the ATP-binding sites of human multidrug resistance P-glycoprotein exposes different residues to the drug-binding site

Loo

Clarke

2002

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

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The human multidrug resistance P-glycoprotein uses ATP to transport a wide variety of structurally unrelated cytotoxic compounds out of the cell. In this study, we used cysteine-scanning mutagenesis and cross-linking studies to identify residues that are exposed to the drug-binding site upon vanadate trapping. In the absence of nucleotides, C222(TM4) was cross-linked to C868(TM10) and C872(TM10); C306(TM5) was cross-linked to C868(TM10), C872(TM10), C945(TM11), C982(TM12), and C984(TM12); and C339(TM6) was cross-linked to C868(TM10), C872(TM10), C942(TM11), C982(TM12), and C985(TM12). These cysteines are in the middle of the predicted transmembrane (TM) segments and form the drug-binding site. Cross-linking between 332C(TM6) and cysteines introduced at the extracellular side of other TM segments was also done. In the absence of nucleotides, residues 332C and 856C on the extracellular side of TMs 6 and 10, respectively, were cross-linked with a 13-Å cross-linker (M8M, 3,6-dioxaoctane-1,8-diyl bismethanethiosulfonate). ATP plus vanadate inhibited cross-linking between 332C(TM6) and 856C(TM10) as well as those in the drug-binding site. Instead, vanadate trapping promoted cross-linking between 332C(TM6) and 976C(TM12) with a 10-Å cross-linker (M6M, 1,6-hexanediyl bismethanethiosulfonate). When ATP hydrolysis was allowed to proceed, then 332C(TM12) could form a disulfide bond with 975C(TM12). The cross-linking pattern of 332C(TM6) with residues in TM10 and TM12 indicates that the drug-binding site undergoes dynamic and relatively large conformational changes, and that different residues are exposed to the drug-binding site during the resting phase, upon vanadate trapping and at the completion of the catalytic cycle.T he human multidrug resistance P-glycoprotein (P-gp) is an ATP-dependent drug pump located at the plasma membrane that can transport a wide variety of structurally diverse compounds of different sizes (recently reviewed in ref. 1). P-gp is clinically important because overexpression of P-gp contributes to the phenomenon of multidrug resistance during treatment of AIDS and cancer. Many of these compounds in these treatment regimens are also substrates of P-gp (2-4). P-gp also plays an important role in mediating the bio-availability of oral drugs because of its relatively higher level of expression in the intestine, brain, liver, and kidney (5-10).P-gp consists of 1,280 aa that are organized in two repeating units of 610 aa that are joined by a linker region of about 60 aa (11). Each repeat has six transmembrane (TM) segments and a hydrophilic domain containing an ATP-binding site (11-13).An important goal in understanding the mechanism of drug transport by P-gp is to determine how ATP hydrolysis is coupled to drug efflux. Both halves of P-gp can hydrolyze ATP (14, 15), but drug-stimulated ATPase activity (14) and conferring of drug resistance (16) requires interaction between the two halves of P-gp. Both halves of P-gp are required for activity because drug binding requires interaction between the NH 2 an...

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Characterization and epitope mapping of several new anti-P-glycoprotein monoclonal antibodies

et al. 1996

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Characterization of the ATPase Activity of Purified Chinese Hamster P-glycoprotein

Cited by 217 publications

References 37 publications

Characterization of the Adenosinetriphosphatase and Transport Activities of Purified Cystic Fibrosis Transmembrane Conductance Regulator

Characterization of the Adenosinetriphosphatase and Transport Activities of Purified Cystic Fibrosis Transmembrane Conductance Regulator

Vanadate trapping of nucleotide at the ATP-binding sites of human multidrug resistance P-glycoprotein exposes different residues to the drug-binding site

Characterization and epitope mapping of several new anti-P-glycoprotein monoclonal antibodies

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