HOME HELP FEEDBACK SUBSCRIPTIONS ARCHIVE SEARCH TABLE OF CONTENTS		QUICK SEARCH:   [advanced] Author: Keyword(s): Year:  Vol:  Page:

This Article Abstract Full Text (PDF) All Versions of this Article: 295/3/C761    most recent 00227.2008v1 Alert me when this article is cited Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via Google Scholar Google Scholar Articles by Silverman, W. Articles by Dahl, G. Search for Related Content PubMed PubMed Citation Articles by Silverman, W. Articles by Dahl, G.

MEMBRANE TRANSPORTERS, ION CHANNELS, AND PUMPS

Probenecid, a gout remedy, inhibits pannexin 1 channels

Department of Physiology and Biophysics, University of Miami School of Medicine, Miami, Florida

Submitted 25 April 2008 ; accepted in final form 29 June 2008

	ABSTRACT

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
Probenecid is a well-established drug for the treatment of gout and is thought to act on an organic anion transporter, thereby affecting uric acid excretion in the kidney by blocking urate reuptake. Probenecid also has been shown to affect ATP release, leading to the suggestion that ATP release involves an organic anion transporter. Other pharmacological evidence and the observation of dye uptake, however, suggest that the nonvesicular release of ATP is mediated by large membrane channels, with pannexin 1 being a prominent candidate. In the present study we show that probenecid inhibited currents mediated by pannexin 1 channels in the same concentration range as observed for inhibition of transport processes. Probenecid did not affect channels formed by connexins. Thus probenecid allows for discrimination between channels formed by connexins and pannexins.

connexin; transport; erythrocyte; ATP release

The inhibitory effect of probenecid on organic anion transporters is well established, and the effect is thought to be so specific that the drug is often used as a diagnostic tool, i.e., its effect is typically interpreted as an involvement of an anion transporter in the tested parameter. Accordingly, block of cAMP or cGMP release from erythrocytes (18, 25), ATP release from glia cells (1, 17), and block of dye loss in various cell types (20, 21, 23) by probenecid have been presented as evidence for a role of transporters in these phenomena. However, alternative pathways for the transit of these molecules across the plasma membrane have to be considered. Besides the well-documented vesicular release of ATP, a parallel release through membrane channels must exist, because the release is attenuated by drugs that do not interfere with vesicular release but affect gap junction proteins and because ATP release in several cell types is associated with uptake of dye from the extracellular medium (13).

Special attention has to be given to pannexin 1 as an ATP release channel because of the specific properties of pannexin 1 channels and because of the expression pattern of pannexin 1 (2, 16, 28, 32–34, 55, 59). Pannexin 1 channels are highly permeable to ATP and to dyes typically used for dye flux measurements through gap junction channels. These dyes are in the same size range as the Ca²⁺ indicator dyes whose loss is attenuated by probenecid. Pannexin 1 channels also are mechanosensitive, consistent with a role in Ca²⁺ wave initiation. Expression of pannexin 1 is found in cells exhibiting ATP release, including erythrocytes, endothelial cells, and astrocytes. Furthermore, the localization at the luminal membrane in epithelial cells is consistent with an ATP release function of pannexin 1 channels.

We therefore tested whether probenecid affects pannexin 1 channels in addition to the drug's action on anion transporters. We also tested the effects of 5-nitro-2(3-phenylpropylamino)-benzoic acid (NPPB) on pannexin 1 channels. NPPB is known as a chloride channel blocker and also has been described to block ATP release from ciliary epithelial cells (36, 45) and mouse mammary cells (47). The results of the present study indicate that probenecid is a powerful inhibitor of pannexin 1 channels. In contrast, connexin channels were not affected by probenecid. NPPB inhibited both pannexin and connexin channels.

	METHODS

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
Preparation of oocytes. Xenopus laevis oocytes were prepared as previously described (15). Briefly, oocytes were isolated by incubating segments of surgically removed ovary in 2 mg/ml collagenase type I (Worthington Biochemical) in Ca²⁺-free oocyte Ringer solution (OR2; in mM: 82.5 NaCl, 2.5 KCl, 1.0 MgCl₂, 1.0 CaCl₂, 1.0 Na₂HPO₄, and 5.0 HEPES, pH 7.5) with antibiotics (10,000 U/ml penicillin and 10 mg/ml streptomycin) and stirring at 1 turn/s for 3 h at room temperature. After being thoroughly washed with regular OR2, oocytes devoid of follicle cells and having a uniform pigmentation were selected and stored in OR2 at 18°C.

mRNA and electrophysiology. mRNA for pannexin 1, connexin46 (Cx46), or Cx32E₁43 were prepared using the mMessage mMachine in vitro transcription kit (Ambion). Oocytes were injected with 20–40 nl of mRNA (100–1,000 ng/ml) and incubated for 18–42 h at 18°C. Oocytes expressing Cx46 or Cx32E₁43 were incubated in OR2 plus 5 mM CaCl₂ to prevent the channels from opening during the incubation. Oocytes were tested using two-electrode voltage clamp (model OC725C, Warner Instruments, or Geneclamp 500B, Axon Instruments) under constant perfusion according to the protocols described. Electrophysiology data are shown as means ± SE or as box plots.

Preparation of erythrocytes. Xenopus blood was collected into OR2 plus 5 mM EGTA, pH 7.5, and spun at low speed. The buffy coat (the thin layer of cells atop the packed erythrocytes) was removed, and erythrocytes were washed three times with OR2 plus 5 mM glucose and then resuspended at 20% hematocrit. Cells were diluted into OR2 without antibiotics for use in dye uptake assays.

Dye uptake. Erythrocytes (75 µl) at 0.1% hematocrit in OR2 were plated onto poly-D-lysine-coated 96-well plates (BioCoat, Becton Dickinson). OR2 alone (25 µl) or with the addition of 4 mM probenecid (Alfa Aesar) was immediately added (final concentration 1 mM), and the cells were allowed to adhere to the plates for 10 min. Solution (50 µl) was removed from the wells, and dye uptake was initiated by the addition of 50 µl of 1.0 mM YoPro-1 iodide (final concentration 0.5 µM) in OR2 (negative control), water (stimulated), or water plus 1.0 mM probenecid (stimulated and inhibited). Images were acquired with a Canon PowerShot S3 IS digital camera with an exposure time of 6 s and an aperture setting of 3.2 attached to the phototube of an inverted fluorescence microscope (model DMIL, Leica).

Extracellular ATP measurements from oocytes. ATP assay solutions (Luciferin/Luciferase, Sigma-Aldrich) were mixed with supernatants collected from pannexin 1-injected and uninjected cells treated with OR2 or potassium gluconate in the presence of 150 or 500 µM probenecid. Oocytes were 4 days postinjection. Pannexin expression and cell viability were confirmed electrophysiologically. Cells were pretreated for 10 min with probenecid, where applicable, and then isolated for 10 min in 150 µl of the experimental solutions. Supernatant (100 µl) was obtained for each condition. Each condition was done in quintuplicate. Luminescence readings were obtained with a Victor 1420 multilabel counter (PerkinElmer) on a 96-well culture plate.

Chemicals. Probenecid [4-(dipropylsulfamoyl)benzoic acid] was obtained from Alfa Aesar. NPPB was obtained from Tocris. NaCl was obtained from EM Science, and CaCl₂ was obtained from J.T.Baker. All other chemicals used were obtained from Sigma-Aldrich.

	RESULTS

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
Pannexin 1, although originally discovered as a "gap junction protein," rather than forming cell-to-cell channels exerts its physiological role as a freestanding, unapposed membrane channel allowing the flux of molecules between the cytoplasm and the extracellular space (2, 8, 9, 12, 16, 28, 39, 42). The channel can be opened at the resting membrane potential by mechanical stress, by an increase in cytoplasmic Ca²⁺ concentration, or by ATP through P2Y or P2X₇ receptors (2, 33, 34). Experimentally, the channel also can be opened by applied voltage pulses (2, 12). The activation of the channel by voltage is probably nonphysiological, because positive potentials are required for the channel to open. However, because of the experimental convenience, we used this paradigm for channel opening.

Figure 1 shows that the organic anion transport inhibitor probenecid attenuates currents induced by voltage steps in pannexin 1-expressing oocytes in a dose-dependant fashion. Figure 2 shows the dose-response curve for the effect of probenecid on pannexin 1 channel currents. At 1 mM concentration, probenecid completely abolished the currents. In the micromolar range, a steep slope for the probenecid effect was observed with an IC₅₀ of 150 µM (Fig. 2). Curiously, at concentrations below 1 µM, a small (<10%) dose-dependent inhibition of the currents was detectable. At these low concentrations, an adaptive phenomenon was observed (Fig. 1B, bottom trace) that was not prominent at higher drug concentrations. Probably there is more than one binding site for probenecid.

View larger version (24K): [in this window] [in a new window]   Fig. 1. Effect of probenecid on pannexin 1-mediated currents. Xenopus oocytes were voltage clamped at a holding potential of –40 mV. Brief voltage steps (5.5 s in duration at a rate of 5 per minute) to +60 mV (top trace) elicited small currents (bottom trace) in uninjected oocytes (A) and significantly larger currents in oocytes injected 2 days before with pannexin 1 mRNA (B and C). The pannexin 1-mediated currents were attenuated by probenecid in a dose-dependent fashion (B). Similarly, 5-nitro-2(3-phenylpropylamino)-benzoic acid (NPPB) attenuated pannexin 1 channel currents (C).

View larger version (9K): [in this window] [in a new window]   Fig. 2. Dose-dependent inhibition of pannexin 1 channel currents by probenecid and NPPB. The dose-response curves for the 2 drugs reveal an IC50 value for probenecid of 150 µM and for NPPB of 50 µM. n = 4 for all data points. For curve fitting and determination of EC50, the submicromolar data points were excluded from the analysis. The Hill slope is 1.2 for probenecid and 0.9 for NPPB. mPanx1, mouse pannexin 1.

To test whether the effects of the two drugs are additive, we applied probenecid and NPPB concurrently, first one drug and then both. Figure 3 shows that at lower concentrations, the effects of the drugs did not add arithmetically. At high concentrations, NPPB left a residual current that remained unaffected by the addition of probenecid at a concentration that abolished the current when given alone. Thus it appears that the drugs act competitively on pannexin 1 channels. A final assessment of the nature of the drug interaction, however, needs to await single-channel studies.

View larger version (15K): [in this window] [in a new window]   Fig. 3. Combined effects of probenecid and NPPB on pannexin 1 channels. Inhibition of the pannexin 1 currents by probenecid was enhanced by the addition of NPPB when both drugs were applied at their IC50 concentrations (A). When given at maximal concentrations, probenecid did not significantly reduce the residual currents in the presence of NPPB (B). A quantitative analysis of the residual currents remaining after application of the drugs at different concentrations (given as IC values) is shown (C). n = 3 for all data points except IC90, where n = 4. *P < 0.05. ns, Not significantly different.

View larger version (19K): [in this window] [in a new window]   Fig. 4. Effect of probenecid and NPPB on connexin 46 (Cx46) and Cx32E143 channels. Oocytes expressing the connexins were held at –30 mV, and depolarizing pulses to –20 mV were applied. The resulting membrane currents are shown. A: probenecid does not affect connexin-based membrane channels. At concentrations exceeding those resulting in total inhibition of pannexin 1 channels, probenecid did not affect currents through Cx46 or Cx32E143 channels. B: currents through Cx46 and Cx32E143 channels were inhibited by NPPB similarly to the pannexin 1 channel currents. Because of different activation kinetics, the oocytes expressing connexins were held at depolarized potentials well below the equilibrium potential for potassium. Therefore, closure of the channels resulted in a considerable baseline shift.

View larger version (7K): [in this window] [in a new window]   Fig. 5. Effects of probenecid and NPPB on Cx46 and Cx32E143 channels. A: both types of channels were unaffected by probenecid (n = 5). B: dose-dependent inhibition of Cx46 channel currents by NPPB. The IC50 for this effect was 50 µM (n = 3).

Erythrocytes from various species, including human, release ATP and take up dye in a low-oxygen environment, when mechanically stressed, or when depolarized with a high concentration of potassium gluconate (6, 32, 50). Figure 6 shows that the osmotic stress-induced uptake of YoPro from the extracellular space by frog erythrocytes was inhibited by probenecid.

View larger version (112K): [in this window] [in a new window]   Fig. 6. Dye uptake by frog erythrocytes. Fluorescence micrographs were taken of the fields shown at 1, 6, and 15 min after application of YoPro, with transmitted light shown at right. When erythrocytes were exposed to the dye YoPro (0.5 µM) in the absence of a stimulus, only a few fluorescent spots were detected (A). Because of their size, these spots probably represent free nuclei. When stimulated by osmotic stress (1:1 diluted oocyte Ringer solution OR2), erythrocytes took up the YoPro as indicated by the intense staining of the nuclei (B). Dye uptake was detectable already within 1 min and increased over time. YoPro uptake was inhibited by 1 mM probenecid (C). Higher magnification of stimulated erythrocytes in a combined bright-field and fluorescence micrograph (D).

View larger version (10K): [in this window] [in a new window]   Fig. 7. ATP release from oocytes expressing pannexin 1. Release of ATP to the extracellular medium by oocytes was measured by luminometry using a luciferase assay. Depolarization of the cells with high-potassium solution (KGlu) resulted in a significant increase in ATP release compared with unstimulated cells. Probenecid attenuated the stimulated release in a dose-dependent way. ATP release from uninjected oocytes is shown at right. Normalized (Norm) luminescence is plotted; n = 7 for all experimental conditions using pannexin 1-expressing oocytes and uninjected oocytes. *P < 0.05. Prob, probenecid.

	DISCUSSION

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

In the present report, however, we show that probenecid inhibits pannexin 1 channels that have no known relationship with transporters. Inhibition of pannexin 1 channels by probenecid has an IC₅₀ of 150 µM, similar to that seen for inhibition of various transporters, including the human urate transporter hURAT1 (10, 46, 54, 57, 58). Considering the established effect on organic anion transport by probenecid, the drug either affects pannexin 1 channels and the transporters as separate entities or pannexin 1 is part of a transport protein complex providing the permeation pathway. In any case, transport claims for many phenomena based on probenecid effects have to be reevaluated in light of the present finding, in particular where a transport process was only inferred from the drug action.

How probenecid accesses and affects the pannexin 1 channel is unclear. Although hydrophobic in nature, the drug is sufficiently water soluble to prepare aqueous stock solutions. The drug, therefore, may interact either with hydrophilic aspects of the protein or may access the channel through the lipid bilayer.

Pannexins were discovered as a second family of vertebrate "gap junction proteins" based on the limited sequence homology to the innexins found in invertebrates (39). However, presently there is no evidence that pannexins actually form gap junction channels in vivo (8, 16, 28, 32, 42). Instead, these proteins seem to exert their physiological role exclusively as nonjunctional membrane channels providing a pathway for exchange of molecules between the cytoplasm and extracellular space (16). Most drugs acting as "gap junction blockers" do not discriminate among connexins, pannexins, and innexins. The only somewhat discriminating agent is carbenoxolone, which requires a slightly lower concentration to affect pannexin channels than connexin channels (11). Probenecid, therefore, is the first drug with specificity for channels formed by pannexins. NPPB is unspecific in its effect on gap junction proteins, as are all the others of the lot, including flufenamic acid, niflumic acid, and higher alcohols.

The inhibitory effect of probenecid on the release of ATP from astrocytes and other cells in the absence of other known targets for the drug has served as evidence for the involvement of transporters in the ATP release mechanism. Because of the strong effect of probenecid on pannexin 1 channels, an involvement of these channels in ATP release has to be seriously considered as an alternative, especially in light of the properties of pannexin 1 channels. They are highly permeable to ATP, activated at the resting membrane potential by mechanical stress, by extracellular ATP through P2Y or P2X₇ receptors, and by increases in cytoplasmic Ca²⁺ concentration (2, 31, 32). Thus pannexin 1 channels are ideally suited to exert the role of ATP release channels in the initiation and propagation of intercellular Ca²⁺ waves. Furthermore, the expression pattern of pannexin 1, including luminal localization, is consistent with such a function.

Additional support for that role also comes from the abundant expression of pannexin 1 in erythrocytes. Erythrocytes release ATP in response to shear stress or in a low-oxygen environment as part of a peripheral control loop of oxygen delivery (6, 50). Under conditions of ATP release, erythrocytes take up dyes from the extracellular medium (32), and as shown in the present study, such dye uptake is inhibited by probenecid. Similarly, ATP release from oocytes expressing pannexin 1 is attenuated by probenecid in the same concentration range as the inhibition of pannexin 1 channel currents. These observations lend further support for a role of the pannexon, the hexameric assembly of pannexins forming a channel (8), as an ATP release channel.

Intercellular Ca²⁺ waves propagate through gap junction channels (48) and by an extracellular pathway involving ATP release and activation of purinergic receptors (27, 38). Typically, this phenomenon is studied with Ca²⁺-sensitive indicator dyes. The dyes are loaded into the cells in the form of membrane permeant esters, which are cleaved by cytoplasmic esterases. Although the cleavage product is essentially membrane impermeant, a gradual loss of dye is observed nevertheless. To prevent dye leakage, it is common practice to use probenecid in these studies with the assumption that the drug will inhibit an organic anion transporter responsible for dye loss (20, 22, 51). This practice has implications and will bias the experimental data toward gap junction-mediated wave propagation because these channels are not affected by probenecid (24). The practice of using probenecid also biases the experimental data toward vesicular release of ATP by attenuating, if not eliminating, pannexin 1-mediated ATP release.

In most cell types, with erythrocytes representing a notable vesicle-free exception, ATP release involves two parallel pathways. There is overwhelming evidence for vesicular release, including copackaging of ATP with other transmitters (49, 53) and sensitivity to Brefeldin (35). A series of observations, however, indicates that an additional, channel-based ATP release mechanism must exist. For example, the dye uptake by cells from the extracellular space under conditions of ATP release cannot be explained by a vesicular release mechanism but is consistent with a channel release process. Furthermore, a series of drugs that do not affect exocytosis attenuate ATP release. Although most of the drugs are not very specific in their action on channels, all of them inhibit pannexin 1 channels, most notably carbenoxolone, probenecid, and NPPB. In summary, these data lend more support for an ATP release channel role for pannexin 1.

Pannexin 1, through its interaction with the P2X₇ receptor, is involved in the activation of the inflammasome, a protein platform that in turn converts interleukin-1β to its releasable form (29, 33, 41). Inflammation is at the root of gout. Thus it appears that probenecid may benefit gout patients in more than one way. In addition to the lowering of systemic uric acid by its action on tubular transport in the kidney, probenecid may stem inflammation through its inhibition of pannexin 1 channels.

	GRANTS

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
This work was supported by National Institutes of Health (NIH) Grant GM-48610 and a NIH Training Grant (to W. Silverman).

	FOOTNOTES

 

Address for reprint requests and other correspondence: G. Dahl, Dept. of Physiology and Biophysics, Univ. of Miami School of Medicine, PO Box 016430, Miami FL 33101 (e-mail: gdahl{at}miami.edu)

The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

	REFERENCES

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
1. Ballerini P, Di Iorio P, Ciccarelli R, Nargi E, D'Alimonte I, Traversa U, Rathbone MP, Caciagli F. Glial cells express multiple ATP binding cassette proteins which are involved in ATP release. Neuroreport 13: 1789–1792, 2002.[CrossRef][Web of Science][Medline]

2. Bao L, Locovei S, Dahl G. Pannexin membrane channels are mechanosensitive conduits for ATP. FEBS Lett 572: 65–68, 2004.[CrossRef][Web of Science][Medline]

3. Bao L, Samuels S, Locovei S, Macagno ER, Muller KJ, Dahl G. Innexins form two types of channels. FEBS Lett 581: 5703–5708, 2007.[CrossRef][Web of Science][Medline]

4. Beahm DL, Hall JE. Hemichannel and junctional properties of connexin 50. Biophys J 82: 2016–2031, 2002.[Web of Science][Medline]

5. Beechwood EC, Berndt WO, Mudge GH. Stop-flow analysis of tubular transport of uric acid in rabbits. Am J Physiol 207: 1265–1272, 1964.[Abstract/Free Full Text]

6. Bergfeld GR, Forrester T. Release of ATP from human erythrocytes in response to a brief period of hypoxia and hypercapnia. Cardiovasc Res 26: 40–47, 1992.[Abstract/Free Full Text]

7. Blomstedt JW, Aronson PS. pH gradient-stimulated transport of urate and p-aminohippurate in dog renal microvillus membrane vesicles. J Clin Invest 65: 931–934, 1980.[Web of Science][Medline]

8. Boassa D, Ambrosi C, Qiu F, Dahl G, Gaietta G, Sosinsky G. Pannexin1 channels contain a glycosylation site that targets the hexamer to the plasma membrane. J Biol Chem 282: 31733–31743, 2007.[Abstract/Free Full Text]

9. Boassa D, Gaietta G, Hu J, Bruzzone R, Dahl G, Sosinsky G. Glycosylation affects plasma membrane targeting of pannexin 1 channels. Am Soc Cell Biol 46th San Francisco B409: 102, 2006.

10. Bobrowska-Hagerstrand M, Wrobel A, Rychlik B, Bartosz G, Soderstrom T, Shirataki Y, Motohashi N, Molnar J, Michalak K, Hagerstrand H. Monitoring of MRP-like activity in human erythrocytes: inhibitory effect of isoflavones. Blood Cells Mol Dis 27: 894–900, 2001.[CrossRef][Web of Science][Medline]

11. Bruzzone R, Barbe MT, Jakob NJ, Monyer H. Pharmacological properties of homomeric and heteromeric pannexin hemichannels expressed in Xenopus oocytes. J Neurochem 92: 1033–1043, 2005.[CrossRef][Web of Science][Medline]

12. Bruzzone R, Hormuzdi SG, Barbe MT, Herb A, Monyer H. Pannexins, a family of gap junction proteins expressed in brain. Proc Natl Acad Sci USA 100: 13644–13649, 2003.[Abstract/Free Full Text]

13. Contreras JE, Sanchez HA, Eugenin EA, Speidel D, Theis M, Willecke K, Bukauskas FF, Bennett MV, Saez JC. Metabolic inhibition induces opening of unapposed connexin 43 gap junction hemichannels and reduces gap junctional communication in cortical astrocytes in culture. Proc Natl Acad Sci USA 99: 495–500, 2002.[Abstract/Free Full Text]

14. Cunningham RF, Israili ZH, Dayton PG. Clinical pharmacokinetics of probenecid. Clin Pharmacokinet 6: 135–151, 1981.[Web of Science][Medline]

15. Dahl G. The Xenopus oocyte cell-cell channel assay for functional analysis of gap junction proteins. In: Cell-Cell Interactions. A Practical Approach, edited by Stevenson B, Gallin W, and Paul D. Oxford: IRL, 1992, p. 143–165.

16. Dahl G, Locovei S. Pannexin: to gap or not to gap, is that a question? IUBMB Life 58: 409–419, 2006.[Web of Science][Medline]

17. Darby M, Kuzmiski JB, Panenka W, Feighan D, MacVicar BA. ATP released from astrocytes during swelling activates chloride channels. J Neurophysiol 89: 1870–1877, 2003.[Abstract/Free Full Text]

18. Davoren PR, Sutherland EW. The effect of L-epinephrine and other agents on the synthesis and release of adenosine 3',5'-phosphate by whole pigeon erythrocytes. J Biol Chem 238: 3009–3015, 1963.[Free Full Text]

19. Deuticke B. Anion permeability of the red blood cell. Naturwissenschaften 57: 172–179, 1970.[CrossRef][Web of Science][Medline]

20. Di Virgilio F, Fasolato C, Steinberg TH. Inhibitors of membrane transport system for organic anions block fura-2 excretion from PC12 and N2A cells. Biochem J 256: 959–963, 1988.[Web of Science][Medline]

21. Di Virgilio F, Steinberg TH, Silverstein SC. Inhibition of fura-2 sequestration and secretion with organic anion transport blockers. Cell Calcium 11: 57–62, 1990.[CrossRef][Web of Science][Medline]

22. Di Virgilio F, Steinberg TH, Silverstein SC. Organic-anion transport inhibitors to facilitate measurement of cytosolic free Ca²⁺ with fura-2. Methods Cell Biol 31: 453–462, 1989.[Web of Science][Medline]

23. Di Virgilio F, Steinberg TH, Swanson JA, Silverstein SC. Fura-2 secretion and sequestration in macrophages. A blocker of organic anion transport reveals that these processes occur via a membrane transport system for organic anions. J Immunol 140: 915–920, 1988.[Abstract]

24. Eugenin EA, Branes MC, Berman JW, Saez JC. TNF-alpha plus IFN-gamma induce connexin43 expression and formation of gap junctions between human monocytes/macrophages that enhance physiological responses. J Immunol 170: 1320–1328, 2003.[Abstract/Free Full Text]

25. Flo K, Hansen M, Orbo A, Kjorstad KE, Maltau JM, Sager G. Effect of probenecid, verapamil and progesterone on the concentration-dependent and temperature-sensitive human erythrocyte uptake and export of guanosine 3',5' cyclic monophosphate (cGMP). Scand J Clin Lab Invest 55: 715–721, 1995.[CrossRef][Web of Science][Medline]

26. Gutman AB. Some recent advances in the study of uric acid metabolism and gout. Bull NY Acad Med 27: 144–164, 1951.[Web of Science][Medline]

27. Hassinger TD, Guthrie PB, Atkinson PB, Bennett MV, Kater SB. An extracellular signaling component in propagation of astrocytic calcium waves. Proc Natl Acad Sci USA 93: 13268–13273, 1996.[Abstract/Free Full Text]

28. Huang Y, Grinspan JB, Abrams CK, Scherer SS. Pannexin1 is expressed by neurons and glia but does not form functional gap junctions. Glia 55: 46–56, 2007.[CrossRef][Web of Science][Medline]

29. Kanneganti TD, Lamkanfi M, Kim YG, Chen G, Park JH, Franchi L, Vandenabeele P, Nunez G. Pannexin-1-mediated recognition of bacterial molecules activates the cryopyrin inflammasome independent of Toll-like receptor signaling. Immunity 26: 433–443, 2007.[CrossRef][Web of Science][Medline]

30. Knickelbein RG, Aronson PS, Dobbins JW. Substrate and inhibitor specificity of anion exchangers on the brush border membrane of rabbit ileum. J Membr Biol 88: 199–204, 1985.[CrossRef][Web of Science][Medline]

31. Lipman BJ, Silverstein SC, Steinberg TH. Organic anion transport in macrophage membrane vesicles. J Biol Chem 265: 2142–2147, 1990.[Abstract/Free Full Text]

32. Locovei S, Bao L, Dahl G. Pannexin 1 in erythrocytes: function without a gap. Proc Natl Acad Sci USA 103: 7655–7659, 2006.[Abstract/Free Full Text]

33. Locovei S, Scemes E, Qiu F, Spray DC, Dahl G. Pannexin1 is part of the pore forming unit of the P2X7 receptor death complex. FEBS Lett 581: 483–488, 2007.[CrossRef][Web of Science][Medline]

34. Locovei S, Wang J, Dahl G. Activation of pannexin 1 channels by ATP through P2Y receptors and by cytoplasmic calcium. FEBS Lett 580: 239–244, 2006.[CrossRef][Web of Science][Medline]

35. Maroto R, Hamill OP. Brefeldin A block of integrin-dependent mechanosensitive ATP release from Xenopus oocytes reveals a novel mechanism of mechanotransduction. J Biol Chem 276: 23867–23872, 2001.[Abstract/Free Full Text]

36. Mitchell CH, Carre DA, McGlinn AM, Stone RA, Civan MM. A release mechanism for stored ATP in ocular ciliary epithelial cells. Proc Natl Acad Sci USA 95: 7174–7178, 1998.[Abstract/Free Full Text]

37. Moller JV. The tubular site of urate transport in the rabbit kidney, and the effect of probenecid on urate secretion. Acta Pharmacol Toxicol (Copenh) 23: 329–336, 1965.[Medline]

38. Osipchuk Y, Cahalan M. Cell-to-cell spread of calcium signals mediated by ATP receptors in mast cells. Nature 359: 241–244, 1992.[CrossRef][Web of Science][Medline]

39. Panchin Y, Kelmanson I, Matz M, Lukyanov K, Usman N, Lukyanov S. A ubiquitous family of putative gap junction molecules. Curr Biol 10: R473–R474, 2000.[CrossRef][Web of Science][Medline]

40. Paul DL, Ebihara L, Takemoto LJ, Swenson KI, Goodenough DA. Connexin46, a novel lens gap junction protein, induces voltage-gated currents in nonjunctional plasma membrane of Xenopus oocytes. J Cell Biol 115: 1077–1089, 1991.[Abstract/Free Full Text]

41. Pelegrin P, Surprenant A. Pannexin-1 mediates large pore formation and interleukin-1beta release by the ATP-gated P2X7 receptor. EMBO J 25: 5071–5082, 2006.[CrossRef][Web of Science][Medline]

42. Penuela S, Bhalla R, Gong XQ, Cowan KN, Celetti SJ, Cowan BJ, Bai D, Shao Q, Laird DW. Pannexin 1 and pannexin 3 are glycoproteins that exhibit many distinct characteristics from the connexin family of gap junction proteins. J Cell Sci 120: 3772–3783, 2007.[Abstract/Free Full Text]

43. Pfahnl A, Zhou XW, Werner R, Dahl G. A chimeric connexin forming gap junction hemichannels. Pflügers Arch 433: 773–779, 1997.[CrossRef][Web of Science][Medline]

44. Pritchard JB, Sweet DH, Miller DS, Walden R. Mechanism of organic anion transport across the apical membrane of choroid plexus. J Biol Chem 274: 33382–33387, 1999.[Abstract/Free Full Text]

45. Reigada D, Lu W, Mitchell CH. Glutamate acts at NMDA receptors on fresh bovine and on cultured human retinal pigment epithelial cells to trigger release of ATP. J Physiol 575: 707–720, 2006.[Abstract/Free Full Text]

46. Roch-Ramel F, Guisan B, Diezi J. Effects of uricosuric and antiuricosuric agents on urate transport in human brush-border membrane vesicles. J Pharmacol Exp Ther 280: 839–845, 1997.[Abstract/Free Full Text]

47. Sabirov RZ, Dutta AK, Okada Y. Volume-dependent ATP-conductive large-conductance anion channel as a pathway for swelling-induced ATP release. J Gen Physiol 118: 251–266, 2001.[Abstract/Free Full Text]

48. Sanderson MJ, Charles AC, Dirksen ER. Mechanical stimulation and intercellular communication increases intracellular Ca²⁺ in epithelial cells. Cell Regul 1: 585–596, 1990.[Web of Science][Medline]

49. Silinsky EM. On the association between transmitter secretion and the release of adenine nucleotides from mammalian motor nerve terminals. J Physiol 247: 145–162, 1975.[Abstract/Free Full Text]

50. Sprague RS, Ellsworth ML, Stephenson AH, Kleinhenz ME, Lonigro AJ. Deformation-induced ATP release from red blood cells requires CFTR activity. Am J Physiol Heart Circ Physiol 275: H1726–H1732, 1998.[Abstract/Free Full Text]

51. Takahashi A, Camacho P, Lechleiter JD, Herman B. Measurement of intracellular calcium. Physiol Rev 79: 1089–1125, 1999.[Abstract/Free Full Text]

52. Ullrich KJ, Rumrich G, Kloss S. Bidirectional active transport of thiosulfate in the proximal convolution of the rat kidney. Pflügers Arch 387: 127–132, 1980.[CrossRef][Web of Science][Medline]

53. Unsworth CD, Johnson RG. Acetylcholine and ATP are coreleased from the electromotor nerve terminals of Narcine brasiliensis by an exocytotic mechanism. Proc Natl Acad Sci USA 87: 553–557, 1990.[Abstract/Free Full Text]

54. Van Aubel RA, Smeets PH, Peters JG, Bindels RJ, Russel FG. The MRP4/ABCC4 gene encodes a novel apical organic anion transporter in human kidney proximal tubules: putative efflux pump for urinary cAMP and cGMP. J Am Soc Nephrol 13: 595–603, 2002.[Abstract/Free Full Text]

55. Vogt A, Hormuzdi SG, Monyer H. Pannexin1 and pannexin2 expression in the developing and mature rat brain. Brain Res Mol Brain Res 141: 113–120, 2005.[Medline]

56. Wright KM, Davies TGE, Steele SH, Leigh RA, Oparka KJ. Development of a probenecid-sensitive Lucifer yellow transport system in vacuolating oat aleurone protoplasts. J Cell Sci 102: 133–139, 1992.[Abstract/Free Full Text]

57. Yamada H, Kotaki H, Itoh T, Sawada Y, Iga T. Effect of anti-inflammatory bowel disease drug, E3040, on urate transport in rat renal brush border membrane vesicles. Eur J Pharmacol 406: 45–48, 2000.[CrossRef][Web of Science][Medline]

58. Yu Z, Fong WP, Cheng CH. Morin (3,5,7,2',4'-pentahydroxyflavone) exhibits potent inhibitory actions on urate transport by the human urate anion transporter (hURAT1) expressed in human embryonic kidney cells. Drug Metab Dispos 35: 981–986, 2007.[Abstract/Free Full Text]

59. Zoidl G, Petrasch-Parwez E, Ray A, Meier C, Bunse S, Habbes HW, Dahl G, Dermietzel R. Localization of the pannexin1 protein at postsynaptic sites in the cerebral cortex and hippocampus. Neuroscience 146: 9–16, 2007.[CrossRef][Web of Science][Medline]

This article has been cited by other articles:

				G. A. Ransford, N. Fregien, F. Qiu, G. Dahl, G. E. Conner, and M. Salathe Pannexin 1 Contributes to ATP Release in Airway Epithelia Am. J. Respir. Cell Mol. Biol., November 1, 2009; 41(5): 525 - 534. [Abstract] [Full Text] [PDF]

				M. Lamkanfi, R. K. S. Malireddi, and T.-D. Kanneganti Fungal Zymosan and Mannan Activate the Cryopyrin Inflammasome J. Biol. Chem., July 31, 2009; 284(31): 20574 - 20581. [Abstract] [Full Text] [PDF]

				W. R. Silverman, J. P. de Rivero Vaccari, S. Locovei, F. Qiu, S. K. Carlsson, E. Scemes, R. W. Keane, and G. Dahl The Pannexin 1 Channel Activates the Inflammasome in Neurons and Astrocytes J. Biol. Chem., July 3, 2009; 284(27): 18143 - 18151. [Abstract] [Full Text] [PDF]

				W. Ma, H. Hui, P. Pelegrin, and A. Surprenant Pharmacological Characterization of Pannexin-1 Currents Expressed in Mammalian Cells J. Pharmacol. Exp. Ther., February 1, 2009; 328(2): 409 - 418. [Abstract] [Full Text] [PDF]

				F. Qiu and G. Dahl A permeant regulating its permeation pore: inhibition of pannexin 1 channels by ATP Am J Physiol Cell Physiol, February 1, 2009; 296(2): C250 - C255. [Abstract] [Full Text] [PDF]

				G. R. Dubyak Both sides now: multiple interactions of ATP with pannexin-1 hemichannels. Focus on "A permeant regulating its permeation pore: inhibition of pannexin 1 channels by ATP" Am J Physiol Cell Physiol, February 1, 2009; 296(2): C235 - C241. [Full Text] [PDF]

This Article Abstract Full Text (PDF) All Versions of this Article: 295/3/C761    most recent 00227.2008v1 Alert me when this article is cited Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via Google Scholar Google Scholar Articles by Silverman, W. Articles by Dahl, G. Search for Related Content PubMed PubMed Citation Articles by Silverman, W. Articles by Dahl, G.