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1.
Measurement of the transport parameters that govern the passage of urea and amides across the red cell membrane leads to
important questions about transport of water. It had initially been thought that small protein channels, permeable to water
and small solutes, traversed the membrane (see Solomon, 1987). Recently, however, very strong evidence has been presented that the 28 kDa protein, CHIP28, found in the
red cell membrane, is the locus of the water channel (see Agre et al., 1993). CHIP28 transports water very rapidly but does not transport small nonelectrolytes such as urea.
The irreversible thermodynamic parameter, σ
i
, the reflection coefficient, is a measure of the relationship between the permeability of the solute and that of water. If
a solute permeates by dissolution in the membrane, σ
i
= 1.0; if it permeates by passage through an aqueous channel, σ
i
< 1.0. For urea, Goldstein and Solomon (1960) found that σurea= 0.62 ± 0.03 which meant that urea crosses the red cell membrane in a water-filled channel. This result and many subsequent
observations that showed that σurea < 1.0 are at variance with the observation that CHIP28 is impermeable to urea.
In view of this problem, we have made a new series of measurements of σ
i
for urea and other small solutes by a different method, which obviates many of the criticisms Macey and Karan (1993) have
made of our earlier method. The new method (Chen et al., 1988), which relies upon fluorescence of the intracellular dye, fluorescein
sulfonate, leads to the corrected value, σurea,corr= 0.64 ± 0.03 for ghosts, in good agreement with earlier data for red cells. Thus, the conclusion on irreversible thermodynamic
and other grounds that urea and water share a common channel is in disagreement with the view that CHIP28 provides the sole
channel for water entrance into the cell.
Received: 6 February 1996/Revised: 20 May 1996 相似文献
2.
R. Novakova D. Homerova R.K.H. Kinne E. Kinne-Saffran J.T. Lin 《The Journal of membrane biology》2001,184(1):55-60
In order to define potential interaction sites of SGLT1 with the transport inhibitor phlorizin, mutagenesis studies were
performed in a hydrophobic region of loop 13 (aa 604–610), located extracellularly, close to the C-terminus. COS 7 cells were
transiently transfected with the mutants and the kinetic parameters of α-methyl-d-glucopyranoside (AMG) uptake into the cells were investigated. Replacement of the respective amino acids with lysine reduced
the maximal uptake rate: Y604K showed 2.2%, L606K 48.4%, F607K 15.1%, C608K 13.1%, G609K 14.1%, and L610K 17.2% of control.
In all mutants the apparent K
i
for phlorizin increased at least by a factor of 5 compared to the wild-type K
i
of 4.6 ± 0.7 μmol/l; most striking changes were observed for Y604K (K
i
= 75.3 ± 19.0 μmol/l) and C608K (K
i
= 83.6 ± 13.9 μmol/l). Replacement of these amino acids with a nonpolar amino acid instead of lysine such as in Y604F, Y604G
and C608A showed markedly higher affinities for phlorizin. In cells expressing the mutants the apparent affinity of AMG uptake
for the sugar was not statistically different from that of the wild type (K
m
= 0.8 ± 0.2 mmol/l).
These studies suggest that the region between amino acids 604 and 610 is involved in the interaction between SGLT1 and phlorizin,
probably by providing a hydrophobic pocket for one of the aromatic rings of the aglucone moiety of the glycoside.
Received: 29 March 2001/Revised: 15 June 2001 相似文献
3.
Nigericin is an ionophore commonly used at the end of experiments to calibrate intracellularly trapped pH-sensitive dyes.
In the present study, we explore the possibility that residual nigericin from dye calibration in one experiment might interfere
with intracellular pH (pH
i
) changes in the next. Using the pH-sensitive fluorescent dye 2′,7′-bis(carboxyethyl)-5,6-carboxyfluorescein (BCECF), we measured
pH
i
in cultured rat renal mesangial cells. Nigericin contamination caused: (i) an increase in acid loading during the pH
i
decrease elicited by removing extracellular Na+, (ii) an increase in acid extrusion during the pH
i
increase caused by elevating extracellular [K+], and (iii) an acid shift in the pH
i
dependence of the background intracellular acid loading unmasked by inhibiting Na-H exchange with ethylisopropylamiloride
(EIPA). However, contamination had no effect on the pH
i
dependence of Na-H exchange, computed by adding the pH
i
dependencies of total acid extrusion and background acid loading. Nigericin contamination can be conveniently minimized by
using a separate line to deliver nigericin to the cells, and by briefly washing the tubing with ethanol and water after each
experiment.
Received: 14 October 1998/Revised: 2 March 1999 相似文献
4.
Electrical breakdown of erythrocytes induces hemoglobin release which increases markedly with decreasing conductivity of
the pulse medium. This effect presumably results from the transient, conductivity-dependent deformation forces (elongation
or compression) on the cell caused by Maxwell stress. The deformation force is exerted on the plasma membrane of the cell,
which can be viewed as a transient dipole induced by an applied DC electric field pulse. The induced dipole arises from the
free charges that accumulate at the cell interfaces via the Maxwell-Wagner polarization mechanism. The polarization response
of erythrocytes to a DC field pulse was estimated from the experimental data obtained by using two complementary frequency-domain
techniques. The response is very rapid, due to the highly conductive cytosol. Measurements of the electrorotation and electrodeformation
spectra over a wide conductivity range yielded the information and data required for the calculation of the deformation force
as a function of frequency and external conductivity and for the calculation of the transient development of the deformation
forces during the application of a DC-field pulse. These calculations showed that (i) electric force precedes and accompanies
membrane charging (up to the breakdown voltage) and (ii) that under low-conductivity conditions, the electric stretching force
contributes significantly to the enlargement of ``electroleaks' in the plasma membrane generated by electric breakdown.
Received: 12 December 1997/Revised: 13 March 1998 相似文献
5.
Zvyagilskaya R Parchomenko O Abramova N Allard P Panaretakis T Pattison-Granberg J Persson BL 《The Journal of membrane biology》2001,183(1):39-50
In this study we have used a newly isolated Yarrowia lipolytica yeast strain with a unique capacity to grow over a wide pH range (3.5–10.5), which makes it an excellent model system for
studying H+- and Na+-coupled phosphate transport systems. Even at extreme growth conditions (low concentrations of extracellular phosphate, alkaline
pH values) Y. lipolytica preserved tightly-coupled mitochondria with the fully competent respiratory chain containing three points of energy conservation.
This was demonstrated for the first time for cells grown at pH 9.5–10.0. In cells grown at pH 4.5, inorganic phosphate (Pi) was accumulated by two kinetically discrete H+/Pi-cotransport systems. The low-affinity system is most likely constitutively expressed and operates at high Pi concentrations. The high-affinity system, subjected to regulation by both extracellular Pi availability and intracellular polyphosphate stores, is mobilized during Pi-starvation. In cells grown at pH 9.5–10, Pi uptake is mediated by several kinetically discrete Na+-dependent systems that are specifically activated by Na+ ions and insensitive to the protonophore CCCP. One of these, a low-affinity transporter operative at high Pi concentrations is kinetically characterized here for the first time. The other two, high-affinity, high-capacity systems,
are derepressible and functional during Pi-starvation and appear to be controlled by extracellular Pi. They represent the first examples of high-capacity, Na+-driven Pi transport systems in an organism belonging to neither the animal nor bacterial kingdoms. The contribution of the H+- and Na+-coupled Pi transport systems in Y. lipolytica cells grown at different pH values was quantified. In cells grown at pH values of 4.5 and 6.0, the H+-coupled Pi transport systems are predominant. The contribution of the Na+/Pi cotransport systems to the total cellular Pi uptake activity is progressively increased with increasing pH, reaching its maximum at pH 9 and higher.
Received: 15 December 2000/Revised: 14 May 2001 相似文献
6.
Voltage-clamp experiments were performed on single bovine adrenal fasciculata cells in short-term primary culture using either
standard (broken membrane) or perforated whole-cell patch clamp recording. The membrane current measured with the perforated
method was dominated by a very stable transient outward current. By contrast, the transient outward current recorded using
the standard method was unstable. The reversal potential of the transient outward current varied linearly with the logarithm
of [K+]
e
with a slope of 47 mV per decade. The onset of activation was sigmoidal and was fitted with a power function where n= 4. Time constants ranged from 1 to 4 msec with a maximum at −25 mV. The steady-state activation curve spanned the voltage
range −50 to +80 mV without reaching a clear maximum. During a pulse, the current decayed in a biexponential manner. Time
constants τ1 and τ2 were voltage-dependent and ranged from 50 to 200 msec respectively for a voltage step at +50 mV. The steady-state inactivation
was dependent on the conditioning pulse duration. Using short conditioning pulses (1.2 sec), the curve which spanned the voltage
range −40 to −20 mV, was 15 mV more positive than that obtained with longer conditioning pulses (60 sec). Time constants of
this ``very slow inactivation' process (τvs) determined for voltage steps at −60 and −50 mV were 15 and 10 sec respectively. A ``facilitation process' of the peak current
was observed when the duration or the amplitude of conditioning pulses were increased in the voltage range −100 to −50 mV.
Recovery from inactivation followed a biexponential time course which seemed a mixture of both inactivation processes. In
some experimental conditions, isolated cells were able to produce overshooting action potentials. These results are discussed
in relation with the membrane electrogenesis of this cell type.
Received: 14 November 1994/Revised: 24 October 1995 相似文献
7.
We characterized the signaling and ion transport pathways that mediate epidermal growth factor receptor physiological control
in SV40-immortalized rabbit corneal epithelial cells (tRCEC). Our evaluation employed single-cell fluorescence imaging to
measure the intracellular [Na+]i in these cells loaded with the Na+ sensitive dye, SBFI. EGF (1 to 5 ng/ml) transiently increased [Na+]i from 10 mm to as much as 35 mm after 25 min, which was followed by a decline towards its control value. These increases waned at higher EGF concentrations
up to 50 ng/ml. Both inhibition of EGF receptor-linked tyrosine kinase activity (50 μm RG-13022) and cPLA2 activity (10 μm AACOCF3) obviated EGF-induced increases in [Na+]i. In contrast, PGE2 (10 μg/ml) and cAMP (2 mm) increased [Na+]i by 25 mm. Inhibition of NKCC activity through exposure to either Cl-free Ringers or 300 μm furosemide in NaCl Ringers eliminated EGF-induced increases in [Na+]i. Similarly, EGF failed to increase [Na+]i following inhibition of: 1) PKA activity (10 μm H-89); 2) Erk1/2 (15 μm PD98059) or 3) p38 (15 μm SB203580) activity. Stimulation protein kinase C activity (0.1 μm PMA) transiently increased [Na+]i followed by a decline towards its baseline value. EGF-induced increases in [Na+]i were unaltered by inhibition of K+ conductance (100 μm 4-AP). Taken together, EGF stimulates Erk1/2; p38 and cPLA2 activity. Their stimulation increases PGE2 and cAMP levels resulting in PKA and NKCC activation.
Received: 18 December 2000/Revised: 24 May 2001 相似文献
8.
Cl− currents (I
Cl) were measured in short fibers (1–2 mm) from the lumbricalis muscle of toads (Bufo arenarum) with two microelectrodes (15°C). Initially the fibers were equilibrated in a high K+-containing solution: (mm) K2SO4 68; Na2SO4 20; KCl 60; CaSO4 8; MgSO4 1; HEPES 2.5. Constant pulses were applied when all the external K+ was replaced by Cs+: Cs2SO4 68; Na2SO4 20; CsCl 60; CaSO4 8; HEPES 2.5 (pH 7.5). Under these conditions about 80–90% of the current is carried by Cl−. The current-voltage relation is almost linear implying constant conductance and hence voltage-independent permeability.
The voltage dependence of the net Cl− current could be fitted by constant field equation with a P
Cl of 3.3 × 10−6 cm/sec. In a separate group of experiments a two-pulse technique was used to estimate the availability and the inactivation
of the initial I
Cl during a test pulse. After returning the potential to the holding potential for various times, test pulses of the same amplitude
and duration of the prepulses were applied. The initial current during the test pulse was 70% of the initial current during
the prepulse and the recovery was complete in less than 300 msec with a linear relationship between the current during the
test pulse and the amplitude of the preceding prepulse. When the test pulses were preceded by a positive prepulse, the initial
current for any given test pulse was larger than with a negative prepulse. If we assumed that the initial current during the
test pulse is a measure of the number of channels open at the end of the prepulse, these results suggest that hyperpolarizing
pulses inactivate and depolarizing prepulses activate the I
Cl.
Received: 31 March 1995/Revised: 27 October 1995 相似文献
9.
In frog red blood cells, K-Cl cotransport (i.e., the difference between ouabain-resistant K fluxes in Cl and NO3) has been shown to mediate a large fraction of the total K+ transport. In the present study, Cl−-dependent and Cl−-independent K+ fluxes via frog erythrocyte membranes were investigated as a function of external and internal K+ ([K+]
e
and [K+]
i
) concentration. The dependence of ouabain-resistant Cl−-dependent K+ (86Rb) influx on [K+]
e
over the range 0–20 mm fitted the Michaelis-Menten equation, with an apparent affinity (K
m
) of 8.2 ± 1.3 mm and maximal velocity (V
max
) of 10.4 ± 1.6 mmol/l cells/hr under isotonic conditions. Hypotonic stimulation of the Cl−-dependent K+ influx increased both K
m
(12.8 ± 1.7 mm, P < 0.05) and V
max
(20.2 ± 2.9 mmol/l/hr, P < 0.001). Raising [K+]
e
above 20 mm in isotonic media significantly reduced the Cl−-dependent K+ influx due to a reciprocal decrease of the external Na+ ([Na+]
e
) concentration below 50 mm. Replacing [Na+]
e
by NMDG+ markedly decreased V
max
(3.2 ± 0.7 mmol/l/hr, P < 0.001) and increased K
m
(15.7 ± 2.1 mm, P < 0.03) of Cl−-dependent K+ influx. Moreover, NMDG+ Cl substitution for NaCl in isotonic and hypotonic media containing 10 mm RbCl significantly reduced both Rb+ uptake and K+ loss from red cells. Cell swelling did not affect the Na+-dependent changes in Rb+ uptake and K+ loss. In a nominally K+(Rb+)-free medium, net K+ loss was reduced after lowering [Na+]
e
below 50 mm. These results indicate that over 50 mm [Na+]
e
is required for complete activation of the K-Cl cotransporter. In nystatin-pretreated cells with various intracellular K+, Cl−-dependent K+ loss in K+-free media was a linear function of [K+]
i
, with a rate constant of 0.11 ± 0.01 and 0.18 ± 0.008 hr−1 (P < 0.001) in isotonic and hypotonic media, respectively. Thus K-Cl cotransport in frog erythrocytes exhibits a strong asymmetry
with respect to transported K+ ions. The residual, ouabain-resistant K+ fluxes in NO3 were only 5–10% of the total and were well fitted to linear regressions. The rate constants for the residual influxes were
not different from those for K+ effluxes in isotonic (∼0.014 hr−1) and hypotonic (∼0.022 hr−1) media, but cell swelling resulted in a significant increase in the rate constants.
Received: 19 November 1998/Revised: 23 August 1999 相似文献
10.
We had previously shown that an influx of extracellular Ca2+ (Ca2+
e
), though it occurs, is not strictly required for aminoethyldextran (AED)-triggered exocytotic membrane fusion in Paramecium. We now analyze, by quenched-flow/freeze-fracture, to what extent Ca2+
e
contributes to exocytotic and exocytosis-coupled endocytotic membrane fusion, as well as to detachment of ``ghosts' — a
process difficult to analyze by any other method or in any other system. Maximal exocytotic membrane fusion (analyzed within
80 msec) occurs readily in the presence of [Ca2+]
e
≥ 5 × 10−6
m, while normally a [Ca2+]
e
= 0.5 mm is in the medium. A new finding is that exocytosis and endocytosis is significantly stimulated by increasing [Ca2+]
e
even beyond levels usually available to cells. Quenching of [Ca2+]
e
by EGTA application to levels of resting [Ca2+]
i
or slightly below does reduce (by ∼50%) but not block AED-triggered exocytosis (again tested with 80 msec AED application).
This effect can be overridden either by increasing stimulation time or by readdition of an excess of Ca2+
e
. Our data are compatible with the assumption that normally exocytotic membrane fusion will include a step of rapid Ca2+-mobilization from subplasmalemmal pools (``alveolar sacs') and, as a superimposed step, a Ca2+-influx, since exocytotic membrane fusion can occur at [Ca2+]
e
even slightly below resting [Ca2+]
i
. The other important conclusion is that increasing [Ca2+]
e
facilitates exocytotic and endocytotic membrane fusion, i.e., membrane resealing. In addition, we show for the first time
that increasing [Ca2+]
e
also drives detachment of ``ghosts' — a novel aspect not analyzed so far in any other system. According to our pilot calculations,
a flush of Ca2+, orders of magnitude larger than stationary values assumed to drive membrane dynamics, from internal and external sources,
drives the different steps of the exo-endocytosis cycle.
Received: 27 September 1996/Revised: 11 February 1997 相似文献
11.
Depolarization-activated H+-selective currents were studied using whole-cell and excised-patch voltage clamp methods in human monocytic leukemia THP-1
cells, before and after being induced by phorbol ester to differentiate into macrophage-like cells. The H+ conductance, g
H, activated slowly during depolarizing pulses, with a sigmoidal time course. Fitted by a single exponential following a delay,
the activation time constant, τact was roughly 10 sec at threshold potentials, decreasing at more positive potentials. Tail currents upon repolarization decayed
mono-exponentially at all potentials. The tail current time constant, τtail, was voltage dependent, decreasing with hyperpolarization from 2–3 sec at 0 mV to ∼200 msec at −100 mV. Surprisingly, although
τact depended strongly on pH
o
, τtail was completely independent of pH
o
. H+ currents were inhibited by Zn2+. Increasing pH
o
or decreasing pH
i
shifted the voltage-activation relationship to more negative potentials, tending to activate the g
H at any given voltage. Studied in excised, inside-out membrane patches, H+ currents were larger and activated much more rapidly at lower bath pH (i.e., pH
i
). In THP-1 cells differentiated into macrophages, the H+ current density was reduced by one-half, and τact was slower by about twofold. The properties of H+ channels in THP-1 cells and in other macrophage-related cells are compared.
Received: 19 September 1995/Revised: 14 March 1996 相似文献
12.
Extracellular nucleotides modulate renal ion transport. Our previous results in M-1 cortical collecting duct cells indicate
that luminal and basolateral ATP via P2Y2 receptors stimulate luminal Ca2+-activated Cl− channels and inhibit Na+ transport. Here we address the mechanism of ATP-mediated inhibition of Na+ transport. M-1 cells had a transepithelial voltage (V
te
) of −31.4 ± 1.3 mV and a transepithelial resistance (R
te
) of 1151 ± 28 Ωcm2. The amiloride-sensitive short circuit current (I
sc
) was −28.0 ± 1.1 μA/cm2. The ATP-mediated activation of Cl− channels was inhibited when cytosolic Ca2+ increases were blocked with cyclopiazonic acid (CPA). Without CPA the ATP-induced [Ca2+]i increase was paralleled by a rapid and transient R
te
decrease (297 ± 51 Ωcm2). In the presence of CPA, basolateral ATP led to an R
te
increase by 144 ± 17 Ωcm2 and decreased V
te
from −31 ± 2.6 to −26.6 ± 2.5 mV. I
sc
dropped from −28.6 ± 2.4 to −21.6 ± 1.9 μA/cm2. Similar effects were observed with luminal ATP. In the presence of amiloride, ATP was without effect. This reflects ATP-mediated
inhibition of Na+ absorption. Lowering [Ca2+]i by removal of extracellular Ca2+ did not alter the ATP effect. PKC inhibition or activation were without effect. Na+ absorption was activated by pHi alkalinization and inhibited by pHi acidification. ATP slightly acidified M-1 cells by 0.05 ± 0.005 pH units, quantitatively not explaining the ATP-induced effect.
In summary this indicates that extracellular ATP via luminal and basolateral P2Y2 receptors inhibits Na+ absorption. This effect is not mediated via [Ca2+]i, does not involve PKC and is to a small part mediated via intracellular acidification.
Received: 9 February 2001/Revised: 17 May 2001 相似文献
13.
Hyperthermia induces transient changes in [Na+]
i
and [K+]
i
in mammalian cells. Since Cl− flux is coupled with Na+ and K+ in several processes, including cell volume control, we have measured the effects of heat on [Cl−]
i
using the chloride indicator, MQAE, with flow cytometry. The mean basal level of [Cl−]
i
in Chinese hamster ovary cells was 12 mm. Cells heated at 42.0° or 45.0°C for 30 min had about a 2.5-fold increase in [Cl−]
i
above unheated control values when measured immediately after heating. There was about a 3-fold decrease in [Na+]
i
under the same conditions, as measured by Sodium Green. The magnitude of the increase in [Cl−]
i
depended upon time and temperature. The [Cl−]
i
recovered in a time-dependent fashion to control values by 30 min after heating. When cells were heated at 45.0°C for 30
min in the presence of 1.5 mm furosemide, the heat-induced [Cl−]
i
increase was completely blocked. Since furosemide inhibits the Na+/K+/2Cl− cotransporter, Cl− channels, and even Cl−HCO3 exchange, these ion transporters may be involved in the heat-induced increase in [Cl−]
i
.
Received: 15 June 1995/Revised: 9 April 1996 相似文献
14.
Davis BA Hogan EM Cooper GJ Bashi E Zhao J Boron WF 《The Journal of membrane biology》2001,183(1):25-32
Previous squid-axon studies identified a novel K/HCO3 cotransporter that is insensitive to disulfonic stilbene derivatives. This cotransporter presumably responds to intracellular
alkali loads by moving K+ and HCO−
3 out of the cell, tending to lower intracellular pH (pHi). With an inwardly directed K/HCO3 gradient, the cotransporter mediates a net uptake of alkali (i.e., K+ and HCO−
3 influx). Here we test the hypothesis that intracellular quaternary ammonium ions (QA+) inhibit the inwardly directed cotransporter by interacting at the intracellular K+ site. We computed the equivalent HCO−
3 influx (J
HCO3) mediated by the cotransporter from the rate of pHi increase, as measured with pH-sensitive microelectrodes. We dialyzed axons to pHi 8.0, using a dialysis fluid (DF) free of K+, Na+ and Cl−. Our standard artificial seawater (ASW) also lacked Na+, K+ and Cl−. After halting dialysis, we introduced an ASW containing 437 mm K+ and 0.5% CO2/12 mm HCO−
3, which (i) caused membrane potential to become transiently very positive, and (ii) caused a rapid pHi decrease, due to CO2 influx, followed by a slower plateau-phase pHi increase, due to inward cotransport of K+ and HCO−
3. With no QA+ in the DF, J
HCO3 was ∼58 pmole cm−2 sec−1. With 400 mm tetraethylammonium (TEA+) in the DF, J
HCO3 was virtually zero. The apparent K
i
for intracellular TEA+ was ∼78 mm, more than two orders of magnitude greater than that obtained by others for inhibition of K+ channels. Introducing 100 mm inhibitor into the DF reduced J
HCO3 to ∼20 pmole cm−2 sec−1 for tetramethylammonium (TMA+), ∼24 for TEA+, ∼10 for tetrapropylammonium (TPA+), and virtually zero for tetrabutylammonium (TBA+). The apparent K
i
value for TBA+ is ∼0.86 mm. The most potent inhibitor was phenyl-propyltetraethylammonium (PPTEA+), with an apparent K
i
of ∼91 μm. Thus, trans-side quaternary ammonium ions inhibit K/HCO3 influx in the potency sequence PPTEA+ > TBA+ > TPA+ > TEA+≅ TMA+. The identification of inhibitors of the K/HCO3 cotransporter, for which no inhibitors previously existed, will facilitate the study of this transporter.
Received: 21 November 2000/Revised: 14 May 2001 相似文献
15.
In cystic fibrosis airway epithelia, mutation of the CFTR protein causes a reduced response of Cl− secretion to secretagogues acting via cAMP. Using a Ca2+ imaging system, the hypothesis that CFTR activation may permit ATP release and regulate [Ca2+]
i
via a receptor-mediated mechanism, is tested in this study. Application of external nucleotides produced a significant increase
in [Ca2+]
i
in normal (16HBE14o− cell line and primary lung culture) and in cystic fibrosis (CFTE29o− cell line) human airway epithelia. The potency order of nucleotides on [Ca2+]
i
variation was UTP ≫ ATP > UDP > ADP > AMP > adenosine in both cell types. The nucleotide [Ca2+]
i
response could be mimicked by activation of CFTR with forskolin (20 μm) in a temperature-dependent manner. In 16HBE14o− cells, the forskolin-induced [Ca2+]
i
response increased with increasing temperature. In CFTE29o− cells, forskolin had no effect on [Ca2+]
i
at body temperature-forskolin-induced [Ca2+]
i
response in CF cells could only be observed at low experimental temperature (14°C) or when cells were cultured at 26°C instead
of 37°C. Pretreatment with CFTR channel blockers glibenclamide (100 μm) and DPC (100 μm), with hexokinase (0.5 U/mg), and with the purinoceptor antagonist suramin (100 μm), inhibited the forskolin [Ca2+]
i
response. Together, these results demonstrate that once activated, CFTR regulates [Ca2+]
i
by mediating nucleotide release and activating cell surface purinoceptors in normal and CF human airway epithelia.
Received: 3 April 2000/Revised: 30 June 2000 相似文献
16.
17.
C. Jumarie P.G.C. Campbell A. Berteloot M. Houde F. Denizeau 《The Journal of membrane biology》1997,158(1):31-48
109Cd uptake was studied using the highly differentiated TC7 clone of Caco-2 cells as a model of human enterocyte function. Intracellular
accumulation of 0.3 μm
109Cd involved a rapid and a slow uptake phase, which resulted in complete equilibration (t
?= 17.3 ± 1.3 min) with an apparent in-to-out distribution ratio (α
e
) of 11.6 ± 0.8. The amplitude of the rapid phase (U
0) and the rate of the slow phase (V) were similarly reduced in the less differentiated PF11 clone, but comparable α
e
values were observed at equilibrium. In both clones, the t
? and α
e
values increased and decreased, respectively, upon addition of unlabeled Cd to the uptake media. In TC7 cells, 109Cd uptake at 1 min (U
1) was unaffected by Ca concentrations four order of magnitude in excess, but both U
0 and V demonstrated similar sensitivities to unlabeled Cd, Zn and sulfhydryl-reactive agents. Only U
0 disappeared when EDTA was present in the wash solutions. U
1 showed saturation kinetics and the data were found compatible with a model assuming rapid initial Cd binding and transport
through a unique transport protein (K
m
= 3.8 ± 0.7 μm). Cd efflux kinetics demonstrated partial reversibility in EDTA-containing solutions, suggesting that the taken up Cd might
be both tightly and loosely bound to intracellular binding sites. However, the displacement of 109Cd measured at 65 min failed to reveal this heterogeneity: the data were found compatible with a model equation assuming the
presence of one class of high-capacity high-affinity binding sites. We conclude that a slow-transport fast-intracellular binding
mechanism of Cd uptake best accounts for these results and that Cd transport most likely involves a carrier-type of protein
unrelated to Ca absorption.
Received: 19 January 1996/Revised: 23 January 1997 相似文献
18.
An apical membrane ouabain-sensitive H-K exchange and a barium-sensitive basolateral membrane potassium channel are present
in colonic crypt cells and may play a role in both K absorption and intracellular pH (pHi) regulation. To examine the possible interrelationship between apical membrane H-K exchange and basolateral membrane K movement
in rat distal colon in the regulation of pHi, experiments were designed to assess whether changes in extracellular potassium can alter pHi. pHi in isolated rat crypts was determined using microspectrofluorimetric measurements of the pH-sensitive dye BCECF-AM (2′,7′-bis(carboxyethyl-5(6)-carboxy-fluorescein
acetoxy methylester). After loading with the dye, crypts were superfused with a Na-free solution which resulted in a rapid
and reversible fall in pHi (7.36 ± 0.02 to 6.98 ± 0.03). Following an increase in extracellular [K] to 20 mm, in the continued absence of Na, there was a further decrease in pHi (0.20 ± 0.02, P < 0.01). K-induced acidification was blocked both by 2 mm bath barium, a K channel blocker, and by 0.5 mm lumen ouabain. K-induced acidification was also observed when intracellular acidification was induced by a NH4Cl prepulse. These observations suggest that increased basolateral K movement increases intracellular [K] resulting in a decrease
in pHi that is mediated by a ouabain-sensitive apical membrane H,K-ATPase. Our results demonstrate an interrelationship between
basolateral K movement and apical H-K exchange in the regulation of pHi and apical K entry in rat distal colon.
Received: 31 March 1998/Revised: 8 September 1998 相似文献
19.
T. Miyashita H. Tatsumi H. Furuta N. Mori M. Sokabe 《The Journal of membrane biology》2001,182(2):113-122
We identified a Ca2+-sensitive cation channel in acutely dissociated epithelial cells from the endolymphatic sac (ES) of guinea pigs using the
patch-clamp technique. Single-channel recordings showed that the cation channel had a conductance of 24.0 ± 1.3 pS (n= 8) in our standard solution. The relative ionic permeability of the channel was in the order K+= Na+ > Ca2+≫ Cl−. This channel was weakly voltage-dependent but was strongly activated by Ca2+ on the cytosolic side at a concentration of around 1 mm in inside-out excised patches. With cell-attached patches, however, the channel was activated by much lower Ca2+ concentrations. Treatment of the cells, under cell-attached configuration, with ionomycin (10 μm), carbonyl cyanide 3-chlorophenylhydrazone (CCCP, 20 μm), or ATP (1 mm), which increased intracellular Ca2+ concentration ([Ca2+]i), activated the channel at an estimated [Ca2+]i from 0.6 μm to 10 μm. It is suggested that some activators of the channel were deteriorated or washed out during the formation of excised patches.
Based on this Ca2+ sensitivity, we speculated that the channel contributes to the regulation of ionic balance and volume of the ES by absorbing
Na+ under certain pathological conditions that will increase [Ca2+]i. This is the first report of single-channel recordings in endolymphatic sac epithelial cells.
Received: 24 October 2000/Revised: 10 April 2001 相似文献
20.
Caffeine causes a [Ca2+]
i
increase in the cortex of Paramecium cells, followed by spillover with considerable attenuation, into central cell regions. From [Ca2+]rest
i
∼50 to 80 nm, [Ca2+]act
i
rises within ≤3 sec to 500 (trichocyst-free strain tl) or 220 nm (nondischarge strain nd9–28°C) in the cortex. Rapid confocal analysis of wildtype cells (7S) showed only a 2-fold cortical
increase within 2 sec, accompanied by trichocyst exocytosis and a central Ca2+ spread during the subsequent ≥2 sec. Chelation of Ca2+
o
considerably attenuated [Ca2+]
i
increase. Therefore, caffeine may primarily mobilize cortical Ca2+ pools, superimposed by Ca2+ influx and spillover (particularly in tl cells with empty trichocyst docking sites). In nd cells, caffeine caused trichocyst
contents to decondense internally (Ca2+-dependent stretching, normally occurring only after membrane fusion). With 7S cells this usually occurred only to a small
extent, but with increasing frequency as [Ca2+]
i
signals were reduced by [Ca2+]
o
chelation. In this case, quenched-flow and ultrathin section or freeze-fracture analysis revealed dispersal of membrane components
(without fusion) subsequent to internal contents decondensation, opposite to normal membrane fusion when a full [Ca2+]
i
signal was generated by caffeine stimulation (with Ca2+
i
and Ca2+
o
available). We conclude the following. (i) Caffeine can mobilize Ca2+ from cortical stores independent of the presence of Ca2+
o
. (ii) To yield adequate signals for normal exocytosis, Ca2+ release and Ca2+ influx both have to occur during caffeine stimulation. (iii) Insufficient [Ca2+]
i
increase entails caffeine-mediated access of Ca2+ to the secretory contents, thus causing their decondensation before membrane fusion can occur. (iv) Trichocyst decondensation
in turn gives a signal for an unusual dissociation of docking/fusion components at the cell membrane. These observations imply
different threshold [Ca2+]
i
-values for membrane fusion and contents discharge.
Received: 23 May 1997/Revised: 18 August 1997 相似文献