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1

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Luminal ATP induces K+ secretion via a P2Y2 receptor in rat distal colonic mucosa (1998)

Kerstan, D. ; Gordjani, N. ; Nitschke, R. ; [et al.]

Springer

Pflügers Archiv 436 (1998), S. 712-716

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ISSN: 1432-2013

Keywords: Key words ATP ; Distal colon ; Exocrine secretion ; K+ secretion ; Luminal receptors ; P2Y2 receptor ; Rat

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract We have previously investigated, in studies of rat distal colonic mucosa, the effect of ATP added to the basolateral side on ion transport and [Ca2+]i. It was demonstrated that ATP acts via a P2Y1 receptor to increase [Ca2+]i and NaCl secretion. In the present study we investigated the effect of luminally added nucleotides (ATP, UTP) on transepithelial voltage (V te) and resistance (R te) in Ussing chamber experiments on rat distal colonic mucosa. Both nucleotides induced a rapid and transient (within 30 s) change of V te to lumen-positive values (resting V te: –2±1 mV; peak V te after 100 µmol/l ATP: +2.4±1.1 mV) and a decrease of R te from 89.9±10.3 to 83.8±9.1 Ωcm2 (n=10). Similar values were obtained with luminal UTP (n=15). The estimated EC50 values for both nucleotides were approximately 6 µmol/l. The ATP-induced V te effect was nearly completely sensitive to Ba2+. Addition of the K+ channel blocker Ba2+ (1 mmol/l) to the luminal solution reversibly inhibited 77±4% (n=5) of the ATP-induced V te effect. Experiments to identify the respective P2 receptor subtype revealed the following rank order of potency at 500 µmol/l agonist: UTP≥ATP〉〉2-methylthio-ATP=ADP〉〉adenosine〉 AMP〉β,γ-methylene-ATP (n=5). This closely resembles the published rank order for the P2Y2 receptor. Using the reverse-transcriptase polymerase chain reaction (RT-PCR) technique P2Y2 receptor-specific mRNA was detected in total RNA extracted from isolated crypts. In summary these data indicate that luminal ATP and UTP act via a P2Y2 receptor in the luminal membrane of colonic mucosa to elicit a transient K+ secretion.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/s004240050693

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A modified confocal laser scanning microscope allows fast ultraviolet ratio imaging of intracellular Ca2+ activity using Fura-2 (1997)

Nitschke, R. ; Wilhelm, S. ; Borlinghaus, R. ; [et al.]

Springer

Pflügers Archiv 433 (1997), S. 653-663

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ISSN: 1432-2013

Keywords: Key words Confocal microscopy ; Acousto-optic tunable filter ; Fura-2 ; Ratio imaging ; HT29 cells

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract A confocal, ultraviolet laser scanning microscope (LSM) for reliable ratio measurements of localized intracellular Ca2+ gradients using the Ca2+-sensitive dye Fura-2 was developed. In a commercial LSM, the filter wheels for the excitation band-pass filters and the grey filters were replaced by acousto-optic tunable filters (AOTF) for rapid switching (≤1.5 μs) of the ultraviolet (351 and 364 nm) and the visible (457, 476, 488, 514 nm) excitation light. This enabled dual wavelength excitation of Fura-2, or 2’7’-biscarboxyethyl-5(6)-carboxyfluorescein (BCECF) for pH measurements. Changing to a transmitted-light detector of high sensitivity allowed for simultaneous recording of differential interference contrast images of the preparation with the excitation light. The AOTF fine control of the intensity of the excitation light and improvements in the emission detector sensitivity enabled the acquisition of up to 120 ratio pairs of high-quality images from a single cell. The optical capabilities and limitations of the instrument were evaluated with fluorescent beads and dye-loaded cultured cells. Agonist-induced intracellular Ca2+ transients in HT29 cells were recorded to test for the instrument’s ability to measure changes in [Ca2+]i. Ratio z-sections from Fura-2-loaded cells showed an inhomogeneity of the Fura-2 loading with an accumulation of the dye mostly in the mitochondria. We show, as an example of the microscope’s achievable resolution, the spatial and temporal heterogeneity of [Ca2+]i signals in mitochondria and the cytosol in response to agonist-evoked stimulation of HT29 cells. In addition, we show that the lipophilic, membrane-bound Fura-2 derivative Fura-C18, for measurements of near-membrane Ca2+ changes, can be used with this confocal microscope. This new LSM is expected to deepen our understanding of localized [Ca2+]i signals; for example, the nuclear Ca2+ signalling or the [Ca2+]i changes that occur during stimulation of ion secretion in polarized epithelial cells.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/s004240050327

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3

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Regulation and possible physiological role of the Ca2-dependent K+ channel of cortical collecting ducts of the rat (1993)

Hirsch, J. ; Leipziger, J. ; Fröbe, U. ; [et al.]

Springer

Pflügers Archiv 422 (1993), S. 492-498

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ISSN: 1432-2013

Keywords: ATP ; pH ; Voltage dependence ; Volume regulation ; Intracellular Ca2+ ; Patch clamp ; Fura-2

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract In the luminal membrane of rat cortical collecting duct (CCD) a big Ca2+-dependent and a small Ca2+-independent K+ channel have been described. Whereas the latter most likely is responsible for the K+ secretion in this nephron segment, the function of the large-conductance K+ channel is unknown. The regulation of this channel and its possible physiological role were examined with the conventional cell-free and the cell-attached nystatin patch-clamp techniques. Patch-clamp recordings were obtained from the luminal membrane of isolated perfused CCD segments and from freshly isolated CCD cells. Intracellular calcium was measured using the calcium-sensitive dye fura-2. The large-conductance K+ channel was strongly voltage- and calcium-dependent. At 3 μmol/l cytosolic Ca2+ activity it was half-maximally activated. At 1 mmol/l it was neither regulated by cytosolic pH nor by ATP. At 1 μmol/l Ca2+ activity the open probability (P o) of this channel was pH-dependent. At pH 7.0 P o was decreased to 4±2% (n=9) and at pH 8.5 it was increased to 425±52% (n=9) of the control. At this low Ca2+ activity the P o of the channel was reduced by 1 mmol/l ATP to 8±4% (n=6). Cell swelling activated the large-conductance K+ channel (n=14) and hyperpolarized the membrane potential of the cells by 9±1 mV (n=23). Intracellular Ca2+ activity increased after hypotonic stress. This increase depended on the extracellular Ca2+ activity. A possible physiological function of the large-conductance K+ channel in rat CCD cells may be the reduction of the intracellular K+ concentration after cell swelling. Once this channel is activated by increases in the cytosolic Ca2+ activity it can be regulated by changes in cellular pH and ATP.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00375077

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4

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Agonist-induced intracellular Ca2+ transients in HT29 cells (1993)

Nitschke, R. ; Leipziger, J. ; Greger, R.

Springer

Pflügers Archiv 423 (1993), S. 519-526

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ISSN: 1432-2013

Keywords: Carbachol ; Adenosine triphosphate ; Neurotensin ; Fura-2 ; Intracellular Ca2+ ; Ca2+ influx ; Mn2+ ; Verapamil ; Ni2+

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract In the present study we have investigated the mechanism of intracellular Ca2+ activity ([Ca2+]i) changes in HT29 cells induced by adenosine triphosphate (ATP), carbachol (CCH), and neurotensin (NT). [Ca2+]i was measured with the fluorescent Ca2+ indicator fura-2 at the single-cell level or in small cell plaques with high time resolution (1–40Hz). ATP and CCH induced not only a dose-dependent [Ca2+]i peak response, but also changes of the plateau phase. The [Ca2+]i plateau was inversely dependent on the ATP concentration, whereas the CCH-induced [Ca2+]i plateau increased at higher CCH concentrations. NT showed (from 10−10 to 10−7 mol/l) in most cases only a [Ca2+]i spike lasting 2–3 min. The [Ca2+]i plateau induced by ATP (10−6 mol/l) and CCH (10−5 mol/l) was abolished by reducing the Ca2+ activity in the bath from 10−3 to 10−4 mol/l (n=7). In Ca2+-free bathing solution the [Ca2+]i peak value for all three agonists was not altered. Using fura-2 quenching by Mn2+ as an indicator of Ca2+ influx the [Ca2+]i peak was always reached before Mn2+ influx started. Every agonist showed this delayed stimulation of the Ca2+ influx with a lag time of 23±1.5 s (n=15) indicating a similar mechanism in each case. Verapamil (10−6–10−4 mol/l) blocked dose dependently both phases (peak and plateau) of the CCH-induced [Ca2+]i increase. Short pre-incubation with verapamil augmented the effect on the [Ca2+]i peak, whereas no further influence on the plateau was observed. Ni2+ (10−3 mol/l) reduced the plateau value by 70%.

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URL: http://dx.doi.org/10.1007/BF00374950

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Cyclosporin-A-induced effects on the free Ca2+ concentration in LLC-PK1-cells and their mechanisms (2000)

Gordjani, N. ; Epting, T. ; Fischer-Riepe, P. ; [et al.]

Springer

Pflügers Archiv 439 (2000), S. 627-633

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ISSN: 1432-2013

Keywords: Ca2+ Cyclosporin A Fura-2 Kidney LLC-PK1-cells Nephrotoxicity Proximal tubule Signal transduction Tacrolimus

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract. Here we have examined the effects of Cyclosporin A (CyA) on the free intracellular Ca2+ concentration ([Ca2+]i) of LLC-PK1/PKE20 cells to evaluate mechanisms of CyA nephrotoxicity using Fura-2 microspectrofluorometry or digital fluorescence video imaging. The CyA-associated changes were compared to the effects of tacrolimus (Tac), a structurally unrelated immunosuppressant with similar cellular pathways which also causes nephrotoxicity. CyA (EC50: 1 nmol/l, n=16) and Tac (EC50: 1 nmol/l, n=5) caused a concentration-dependent increase of [Ca2+]i which was substantially attenuated by reducing the external Ca2+ concentration (10–6 mol/l). Similarly Cyclosporin H, a non-immunosuppressive analogue of CyA, stimulated a Ca2+ influx. Nicardipine (10–6 mol/l) reduced the CyA- and the Tac-induced Ca2+ influx to 52±16% (n=10) and 13±10% (n=13) of control respectively. Diltiazem and verapamil (10–6 mol/l) were also effective, but flufenamate (10–4 mol/l), Gd3+ (10–5 mol/l) and La3+ (10–5 mol/l) were not. In the absence of extracellular Ca2+ CyA led to a small but significant [Ca2+]i increase, indicating additional release from internal stores. Depletion of inositol-1,4,5-trisphosphate- (InsP 3-) sensitive Ca2+ stores by extracellular ATP (10–4 mol/l) in low-Ca2+ solution completely suppressed the CyA-induced [Ca2+]i rise. CyA had no effect on the cellular InsP 3 concentration. Furthermore, inhibition of phospholipase-Cβ (PLCβ) by U73122 (2×10–5 mol/l) did not alter the CyA-stimulated [Ca2+]i rise. A direct effect of CyA on InsP 3-sensitive Ca2+ stores, the InsP 3 receptor, the Ca2+ content of the stores or involvement of additional stores is assumed. Incubation with CyA for 1, 12 and 24 h enhanced the rise in [Ca2+]i peak induced by ATP, arginine vasopressin (AVP) and angiotensin II. In summary, CyA stimulated a [Ca2+]i increase in LLC-PK1 cells through Ca2+ release from InsP 3-sensitive stores and Ca2+ influx via a nicardipine-sensitive pathway. The CyA-mediated [Ca2+]i increase is independent of PLCβ activity and InsP 3 metabolism. CyA caused long-term enhancement of the agonist-induced rise in [Ca2+]i. The effects of CyA on Ca2+ signaling appear to be independent of its immunosuppressive action.

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URL: http://dx.doi.org/10.1007/s004249900205

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Forskolin and PMA pretreatment of HT29 cells alters their chloride conductance induced by cAMP, Ca2+ and hypotonic cell swelling (1994)

Kunzelmann, K. ; Allert, N. ; Kubitz, R. ; [et al.]

Springer

Pflügers Archiv 428 (1994), S. 76-83

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ISSN: 1432-2013

Keywords: HT29 ; CFPAC-1 ; Cl− secretion ; CFTR ; CF ; Cl− conductance

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract HT29 cells were preincubated with forskolin (10−5 mol/l, FORHT) or phorbol 12-myristate 13-acetate (PMA) (10−7 mol/l, PMAHT) for 20 h, which has been shown previously and is also shown here, to upregulate and downregulate, respectively, the expression of the cystic fibrosis transmembrane conductance regulator (CFTR). CFPAC-1 cells underwent the same protocols. HT29 cells were examined by slow (SWC) and fast (FWC) whole-cell patch-clamp techniques. The results of SWC and FWC were indistinguishable and were pooled. CFPAC-1 cells were examined with FWC. The membrane voltage (V) of FORHT was -41.8±1.4 mV (n=77) and that of PMAHT was -43.6±2.4 mV (n=76). The conductance (G) of FORHT (9.4 ±0.9 nS, n=77) was significantly larger than that of PMAHT (3.7±0.4 nS, n=76). Acute application of forskolin (10−5 mol/l, FOR) plus 0.5 mmol/l 8-(4-chlorophenylthio)-cAMP (cAMP) depolarized V by 12 (FORHT) and 8 (PMAHT) mV, respectively. The acute increase of G by FOR plus cAMP was by 7.6±1.9 nS for FORHT (n=22) and only 2.2±1 nS for PMAHT (n=13). ATP (10−4 mol/l) depolarized V in both types of cells. It enhanced G by 16.7±4.1 nS in FORHT (n=14) and significantly less (by 5.5±1.2nS, n=14) in PMAHT. Also the G increase lasted longer in FORHT. Neurotensin (NT, 10−8 mol/l) also had a stronger and longer lasting effect in FORHT. Exposure to hypotonic bath solution (160 mosmol/l) depolarized V in both types of cells. The increase in G was by 15±2.2 nS in FORHT (n=18) and by 11±1.3 nS in PMAHT (n=23). After being returned to the normotonic media, the decline of G to the control value was delayed in FORHT when compared to PMAHT. Ionomycin (10−7 mol/l) increased G significantly more (to 47±8.5 nS, n=13) in FORHT when compared to PMAHT (to 28±4 nS, n=13). The present data indicate that a 20-h exposure of HT29 cells to FOR versus PMA alters markedly the CFTR concentration. The cells with high CFTR (FORHT) when compared to those with low CFTR (PMAHT) differ not only in their acute G response to cAMP, but also in that to ATP, NT, hypotonic cell swelling, and ionomycin. In contrast, the same pretreatment of CFPAC-1 cells did not alter the G changes induced by ionomycin or hypotonic cell swelling. These results indicate that changes in CFTR expression correlate with the Cl− conductances induced by cAMP, Ca2+ and hypotonic cell swelling.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00374754

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pH regulation in HT29 colon carcinoma cells (1994)

Köttgen, M. ; Leipziger, J. ; Fischer, K. -G. ; [et al.]

Springer

Pflügers Archiv 428 (1994), S. 179-185

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ISSN: 1432-2013

Keywords: BCECF ; Na+/H+ exchanger ; HCO 3 − /Cl− exchanger ; Na+-dependent HCO 3 − transporter ; DIDS ; HOE-694

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract The pH regulation in HT29 colon carcinoma cells has been investigated using the pH-sensitive fluorescent indicator 2′,7′-biscarboxyethyl-5(6)-carboxyfluorescein (BCECF). Under control conditions, intracellular pH (pHi) was 7.21±0.07 (n=22) in HCO 3 − -containing and 7.21±0.09 (n=12) in HCO 3 − -free solution. HOE-694 (10 μmol/l), a potent inhibitor of the Na+/H+ exchanger, did not affect control pHi. As a means to acidify cells we used the NH 4 + /NH3 (20 mmol/l) prepulse technique. The mean peak acidification was 0.37±0.07 pH units (n=6). In HCC 3 − -free solutions recovery from acid load was completely blocked by HOE-694 (1 μmol/l), whereas in HCO3 3 − -containing solutions a combination of HOE-694 and 4,4′-diisothiocyanatostilbene-2, 2′-disulphonate (DIDS, 0.5 mmol/l) was necessary to show the same effect. Recovery from acid load was Na+-dependent in HCO 3 − -containing and HCO 3 − -free solutions. Removal of external Cl− caused a rapid, DIDS-blockable alkalinization of 0.33±0.03 pH units (n=15) and of 0.20±0.006 pH units (n=5), when external Na+ was removed together with Cl−. This alkalinization was faster in HCO 3 − -containing than in HCO 3 − -free solutions. The present observations demonstrate three distinct mechanisms of pH regulation in HT29 cells: (a) a Na+/H+ exchanger, (b) a HCO 3 − /Cl− exchanger and (c) a Na+-dependent HCC 3 − transporter, probably the Na+-HCO 3 − /Cl− antiporter. Under HCO 3 − — free conditions the Na+/H+ exchanger fully accounts for recovery from acid load, whereas in HCO 3 − -containing solutions this is accomplished by the Na+/H+ exchanger and a Na+-dependent mechanism, which imports HCO 3 − . Recovery from alkaline load is caused by the HCO 3 − /Cl− exchanger.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00374856

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cAMP and Ca2+ act co-operatively on the Cl− conductance of HT29 cells (1992)

Allert, N. ; Leipziger, J. ; Greger, R.

Springer

Pflügers Archiv 421 (1992), S. 403-405

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ISSN: 1432-2013

Keywords: HT29 ; CFPAC-1 ; Cl− Secretion ; cAMP ; ATP ; Neurotensin

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract Previous studies in HT29 cells have revealed that the Cl− channels induced by cAMP or by increasing cytosolic Ca2+, e.g. by addition of ATP, and by hypotonic cell swelling share in common all examined properties, such as ion selectivity and blocker sensitivity. In addition, it was shown that conductances induced by either pathway were not additive. Therefore all three pathways apparently act on the same type of small conductance Cl− channel. In CFPAC-1 cells the general properties of the Cl− conductance were identical. However, the cAMP response was absent. In both cell types the Ca2+-mediated conductance response was transient. Here we examine the kinetics of the conductance increases induced by neurotensin (NT, 10−8 mol/l) or ATP (10−5 mol/l) in HT29 and CFPAC-1 cells using the slow (nystatin) or fast whole cell patch clamp technique, and we ask whether cAMP influences these kinetics. In the continuous presence of NT the conductance response in both cell types was very transient. It collapsed with a time constant (τ) of 39 (30–56 s) in HT29 and of 33 (27–41 s) in CFPAC-1 cells. The ATP response was also transient with a τ of 49 (42–57 s) in HT29 cells and 102 (77–152 s) in CFPAC-1 cells. Pre-treatment by membrane permeable cAMP (10−3 mol/l) enhanced the baseline conductance in HT29 but not in CFPAC-1 cells. Furthermore, the ATP- and NT-induced conductance increases became significantly less transient in HT29 but not in CFPAC-1 cells. In the former cells τ was enhanced significantly to 207 (154–316 s) after ATP and to 1.533 (1004-∞ s) after NT. In CFPAC-1 cells the transient nature of the conductance response persisted. These data indicate that cAMP and Ca2+ co-operate in HT29- but not in CFPAC-1-cells. In the former cells the transient conductance response is converted into a more stable response by cAMP. In CFPAC-1 cells the cAMP-mechanism is not functioning. Therefore, all Ca2+-mediated conductance responses are only very transient.

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URL: http://dx.doi.org/10.1007/BF00374233

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Flufenamate and Gd3+ inhibit stimulated Ca2+ influx in the epithelial cell line CFPAC-1 (1994)

Schumann, S. ; Greger, R. ; Leipziger, J.

Springer

Pflügers Archiv 428 (1994), S. 583-589

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ISSN: 1432-2013

Keywords: Ca2+ influx ; Fura-2 ; CFPAC-1 ; Flufenamate ; Gd3+ ; ATP ; Thapsigargin

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract The relevant influx pathway for stimulated Ca2+ entry into epithelial cells is largely unknown. Using flufenamate (Flu) and Gd3+, both known pharmacological blockers of non-selective cation currents in other epithelial preparations, we tested whether the stimulated Ca2+ entry in CFPAC-1 cells was inhibited by these agents. Transmembraneous Ca2+ influx into CFPAC-1 cells was stimulated by either ATP (10−4 and 10−5 mol/l), carbachol (CCH, 10−4 mol/l) or thapsigargin (TG, 10−8 mol/l). Three different experimental approaches were used. (1) Because the plateau phase of an agonist-induced [Ca2+]i transient reflects Ca2+ influx into these cells, we investigated the influence of Flu and Gd3+ on the level of the stimulated [Ca2+]i plateau. (2) The fura-2 Mn2+-quenching technique was used to visualise divalent cation entry and monitor its inhibition. (3) During the “refilling period” after agonist-induced discharge of the intracellular pools the putative influx inhibitors Flu and Gd3+ were given and subsequently the filling state of the agonist-sensitive intracellular stores tested. The results from the first experimental approach showed that both Flu and Gd3+ were potent inhibitors of the stimulated Ca2+ entry in CFPAC-1 cells. Flu reversibly decreased the ATP-induced [Ca2+]i plateau in a concentration dependent manner, with an IC50 value of 33 μmol/l (n = 6). Similar results were obtained for the CCH-(n = 5) and the TG-induced (n = 5) [Ca2+]i plateau. Gd3+ concentration dependently inhibited the stimulated Ca2+ plateau. A complete block of the ATP-induced [Ca2+]i plateau was seen at 0.5 μmol/l (ATP 10−5 mol/l, n = 8). The second approach showed that Flu (10−4 mol/l) completely inhibited the ATP- (10−5 mol/l, n = 3), CCH-(10−4 mol/l, n = 4) and TG-(10−8 mol/l, n = 3)-induced fura-2 Mn2+ quench. Gd3+ also inhibited the fura-2 Mn2+-quenching rate (n = 9). The third approach showed that Flu (n = 6) and Gd3+ (n = 8) inhibited the refilling of the ATP-sensitive intracellular Ca2+ store. These results show that inhibitors of non-selective cation currents in other epithelial preparations are potent inhibitors of stimulated Ca2+ influx in CFPAC-1 cells. Whether this inhibitory effect concerns a non-selective cation channel remains to be established.

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URL: http://dx.doi.org/10.1007/BF00374581

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pH dependence of K+ conductances of rat cortical collecting duct principal cells (1994)

Schlatter, E. ; Haxelmans, S. ; Hirsch, J. ; [et al.]

Springer

Pflügers Archiv 428 (1994), S. 631-640

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ISSN: 1432-2013

Keywords: Intracellular pH ; K+ channel ; NH4 +/NH3 Patch clamp ; BCECF

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract The K+ channels of the principal cells of rat cortical collecting duct (CCD) are pH sensitive in excised membranes. K+ secretion is decreased with increased H+ secretion during acidosis. We examined whether the pH sensitivity of these K+ channels is present also in the intact cell and thus could explain the coupling between K+ and H+ secretion. Membrane voltages (V m), whole-cell conductances (g c), and single-channel currents of K+ channels were recorded from freshly isolated CCD cells or isolated CCD segments with the patch-clamp method. Intracellular pH (pHi) was measured using the pH-sensitive fluorescent dye 2′-7′-bis(carboxyethyl)-5-6-carboxyfluorescein (BCECF). Acetate (20 mmol/l) had no effect on V m, g c, or the activity of the K+ channels in these cells. Acetate, however, acidified pHi slightly by 0.17±0.04 pH units (n=19). V m depolarized by 12±3 mV (n=26) and by 23±2 mV (n=66) and g c decreased by 26±5% (n=13) and by 55±5% (n=12) with 3–5 or 8–10% CO2, respectively. The same CO2 concentrations decreased pHi by 0.49±0.07 (n=15) and 0.73±0.11 pH units (n=12), respectively. Open probability (P o) of all four K+ channels in the intact rat CCD cells was reversibly inhibited by 8–10% CO2. pHi increased with the addition of 20 mmol/l NH4 +/NH3 by a maximum of 0.64±0.08 pH units (n=33) and acidified transiently by 0.37±0.05 pH units (n=33) upon NH4 +/NH3 removal. In the presence of NH4 +/NH3 V m depolarized by 16±2 mV (n=66) and g c decreased by 26±7% (n=16). The activity of all four K+ channels was also strongly inhibited in the presence of NH4 +/NH3. The effect of NH4 +/NH3 on V m and g c was markedly increased when the pH of the NH4 +/NH3-containing solution was set to 8.5 or 9.2. From these data we conclude that cellular acidification in rat CCD principal cells down-regulates K+ conductances, thus reduces K+ secretion by direct inhibition of K+ channel activity. This pH dependence is present in all four K+ channels of the rat CCD. The inhibition of K+ channels by NH4 +/NH3 is independent of changes in pHi and rather involves an effect of NH3.

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URL: http://dx.doi.org/10.1007/BF00374587

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