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: 291/6/L1169    most recent 00117.2006v1 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 ISI Web of Science Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via Google Scholar Google Scholar Articles by Fike, C. D. Articles by Madden, J. A. Search for Related Content PubMed PubMed Citation Articles by Fike, C. D. Articles by Madden, J. A.

Voltage-gated K⁺ channels at an early stage of chronic hypoxia-induced pulmonary hypertension in newborn piglets

Department of Neurology, Medical College of Wisconsin, Milwaukee, Wisconsin; Department of Pediatrics, Vanderbilt University School of Medicine, Nashville, Tennessee; and Department of Pediatrics, Wake Forest University School of Medicine, Winston-Salem, North Carolina

Submitted 29 March 2006 ; accepted in final form 27 June 2006

	ABSTRACT

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
Our purpose was to determine whether smooth muscle cell membrane properties are altered in small pulmonary arteries (SPA) of piglets at an early stage of pulmonary hypertension. Piglets were raised in either room air (control) or hypoxia for 3 days. A microelectrode technique was used to measure smooth muscle cell membrane potential (E_m) in cannulated, pressurized SPA (100- to 300-µm diameter). SPA responses to the voltage-gated K⁺ (K_V) channel antagonist 4-aminopyridine (4-AP) and the K_V1 family channel antagonist correolide were measured. Other SPA were used to assess amounts of K_V1.2, K_V1.5, and K_V2.1 (immunoblot technique). E_m was more positive in SPA of chronically hypoxic piglets than in SPA of comparable-age control piglets. The magnitude of constriction elicited by either 4-AP or correolide was diminished in SPA from hypoxic piglets. Abundances of K_V1.2 were reduced, whereas abundances of both K_V1.5 and K_V2.1 were unaltered, in SPA from hypoxic piglets. At least partly because of reduced amounts of K_V1.2, smooth muscle cell membrane properties are altered such that E_m is depolarized and K_V channel family function is impaired in SPA of piglets at an early stage of chronic hypoxia-induced pulmonary hypertension.

membrane potential; membrane depolarization; K_V1.2; K_V1.5; K_V2.1; 4-aminopyridine; correolide

There is growing evidence that changes in K_V channel function and/or expression along with the concomitant influence on E_m could contribute to pulmonary hypertension in adults (18, 20). Indeed, K_V channel function and expression are altered in PASMC of adult humans with either primary pulmonary hypertension (45) or anorexigen-induced pulmonary hypertension (41). In addition, a number of studies with adult rats have shown that chronic hypoxia impairs PASMC K⁺ channel current (15, 26, 30, 33), decreases PASMC K_V channel expression (15, 26, 30, 39), and depolarizes PASMC (15, 27, 33, 34).

In contrast to the studies in adult animals, the effect of chronic hypoxia on membrane properties of PASMC from newborn animals has received almost no attention (11). Extrapolation of data collected from adults may not be applicable to newborns as the regulation of pulmonary vascular pressure has long been known to be influenced by postnatal age (5, 32, 46). Because of their critical role in regulation of pulmonary vascular tone, the elucidation of PASMC membrane properties in small, resistance-level, pulmonary arteries is of particular importance. We previously showed (12) that pulmonary hypertension develops when newborn pigs are exposed to chronic hypoxia for 3 days and that pulmonary hypertension worsens when hypoxic exposure is extended from 3 to 10 days. The major purpose of this study was to test the hypothesis that in vivo exposure to chronic hypoxia concomitantly depolarizes PASMC E_m and alters K_V channel function and expression in small, resistance-level, pulmonary arteries of newborn piglets. We evaluated changes that occur with 3-day exposure to hypoxia because of the potential significance for developing therapies to intervene at an early stage and prevent progression of pulmonary hypertension.

	METHODS

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
Animals. Newborn pigs (2–3 days old) were placed in a hypoxic normobaric chamber for 3 days. Normobaric hypoxia was produced by delivering compressed air and N₂ to a plastic chamber so that oxygen content was maintained at 10–11% O₂ (PO₂ 60–72 Torr). CO₂ was maintained at 3–6 Torr by absorption with soda lime. Two times per day the chambers were opened, at which time the piglets were cleaned and weighed. The animals were fed ad libitum with an artificial sow milk replacer from a feeding device attached to the chamber. With respect to control pigs, we previously found (12) no differences in vascular responses between piglets raised in a room air environment for 3–4 days and piglets raised on a farm. Therefore, for this study, all but three of the control piglets were studied on the day of arrival from the farm at 5–7 days of age.

On the day of study the piglets were preanesthetized with acepromazine (2 mg/kg im) and ketamine (10 mg/kg im) and then anesthetized with pentobarbital (30 mg/kg iv). All animals were given heparin (1,000 IU/kg iv) and then exsanguinated. The thorax was opened, and the lungs were removed and placed in cold (4°C) physiological saline solution (PSS) until use. The PSS had the following composition (in mM): 141 Na⁺, 4.7 K⁺, 125 Cl^–, 2.5 Ca²⁺, 0.72 Mg²⁺, 1.7 H₂PO₄^–, 25 HCO₃^–, and 11 glucose. All procedures involving animals were approved by the Institutional Animal care and Use Committees at Wake Forest University School of Medicine and Vanderbilt University School of Medicine.

Cannulated artery preparation. Immediately before use, segments of 100- to 300-µm-diameter pulmonary arteries were dissected from a lung lobe. The system used to study cannulated arteries was described in detail previously (14). The exterior of the artery was suffused with PSS from a reservoir at 37°C and aerated with a gas mixture containing 21% O₂, 5% CO₂, and 74% N₂. The arterial lumen was filled from a syringe containing PSS, aerated with the same gas mixture as the reservoir, and connected to the cannula with polyethylene tubing. Gas concentrations and pH were monitored in all solutions with a blood gas analyzer. Inflow pressure was adjusted by changing the height of the reservoir. The artery was observed continuously with a video system containing a color camera (Hitachi VCC151) and a color television monitor. Vessel diameters were measured with a videoscaler (FORA IV).

Cannulated artery and smooth muscle cell E_m determination protocols. All arteries were equilibrated for 30–60 min at transmural pressures that approximated in vivo pressures (12, 13): control arteries were equilibrated at a transmural pressure of 15 cmH₂O, and hypoxic arteries were equilibrated at a transmural pressure of 25 cmH₂O. After equilibration and establishment of basal tone, all arteries were tested for viability by contraction to U-46619 (10^–8 M). The presence of a functional endothelium was determined in control arteries by dilation of the vessel to acetylcholine (ACh, 10^–6 M). We previously found (14) that although hypoxic arteries constricted to ACh they dilated to the calcium ionophore A-23187, which also requires the endothelium for its function as a dilator. Therefore, changes in vessel diameter to A-23187 were used to check for a functional endothelium in hypoxic arteries.

To measure smooth muscle cell (SMC) E_m, techniques described previously were used (1, 17). In brief, arteries from some control and hypoxic piglets were cannulated, pressurized, and equilibrated as described above. SMC were impaled with microelectrodes filled with 3 M KCl and having impedances between 40 and 90 M. The microelectrode was connected to a high-impedance biological amplifier (Dagan) that was attached to a digital data acquisition system (PowerLab from ADI Instruments). With a micromanipulator, the electrode was advanced into a SMC from the adventitial side of the artery. Criteria for a successful impalement included an abrupt drop in potential to a new steady-state value that was maintained for a minimum of 10 s and returned to the original baseline value when the microelectrode was removed from the SMC. Multiple successful impalements of at least three vascular SMC were averaged for a single artery.

To assess the influence of the endothelium, SMC E_m was measured in some arteries from control and hypoxic piglets after the endothelium was disrupted with air infusion. Effective functional disruption of the endothelium was verified by loss of relaxation to ACh and/or A-23817 for the control arteries and by loss of relaxation to A-23187 for the hypoxic arteries. We also evaluated the influence of transmural pressure on SMC E_m. To do this, we measured SMC E_m in some control arteries that were pressurized to the transmural pressure used for hypoxic arteries (25 cmH₂O) and measured SMC E_m in some hypoxic arteries that were pressurized to the transmural pressure used for control arteries (15 cmH₂O).

To evaluate K_V channel function, we measured changes in vessel diameter in response to pharmacological blockade with the K_V channel antagonist 4-aminopyridine (4-AP) in control and hypoxic arteries. For these studies, we continuously monitored the vessel diameter while adding cumulative doses of 4-AP (10^–5–10^–3 M) to the reservoir. In some control and hypoxic arteries, we measured SMC E_m 20–30 min after adding the last dose of 4-AP to the reservoir. The influence of the endothelium on 4-AP responses was assessed by performing studies in other arteries after disrupting the endothelium by air infusion. Effective functional disruption of the endothelium was verified by loss of relaxation to ACh and/or A-23817 for the control arteries and by loss of relaxation to A-23187 for the hypoxic arteries.

The contribution of some other K⁺ channel families to vascular diameter was also assessed by pharmacological blockage. BaCl₂ (10^–4 M) was used to block inwardly rectifying K⁺ (K_ir) channels, and iberiotoxin (10^–7 M) was used to block BK_Ca channels. The K_V1 family of channels was blocked with the specific antagonist correolide (10^–8–10^–6 M). For some vessels, 20–30 min after pharmacological block of the K_V1 channels with correolide, the effect of pharmacological block of all K_V channels with 4-AP (10^–3 M) was measured. Vessel viability was tested at the completion of each study by addition of U-46619. In addition, in some studies vessel responses to the vehicle used for solubilization of each agent were evaluated.

Immunoblot analyses of K_V1.2, K_V1.5, and K_V2.1. Pulmonary arteries (20- to 600-µm diameter) were dissected from lungs of control and hypoxic piglets, frozen in liquid nitrogen, and stored at –80°C until use for immunoblot analysis.

For each protein, we performed preliminary studies with different amounts of total protein to determine the dynamic range of the immunoblot analysis. An amount of protein that was within the dynamic range of the immunoblot analysis for that protein (for K_V1.2 we used 30-µg protein samples; for K_V1.5 analysis we used 20-µg protein samples; for K_V2.1 we used 30-µg protein samples) was then used to compare protein abundance between homogenates of small pulmonary arteries from control and hypoxic piglets as follows.

Frozen samples of small pulmonary arteries (20- to 600-µm diameter) from control (n = 5) and hypoxic (n = 5) piglets were crushed into a fine powder under liquid N₂ in a prechilled mortar and pestle, transferred to a tube containing homogenate buffer, and then sonicated with three 15-s pulses, taking care not to foam the sample. The supernatant was centrifuged, and the protein concentration was determined by protein assay (Bradford). Each vessel homogenate was diluted with phosphate-buffered saline (PBS) to obtain a protein concentration of 1 mg/ml. Aliquots of the protein concentrations were solubilized in equal volumes of denaturing, reducing sample buffer (Novex; 20 mM Tris·HCl, 2.5 mM EDTA, 0.5% Triton X-100, 0.05% SDS, 100 mM NaCl, 1 mM PMSF, 10 ng/ml leupeptin, and 10 µg/ml pepstatin), heated to 80°C for 15 min, and centrifuged for 3 min at 5,600 g in a microfuge. Equal volumes of these supernatants were then applied to Tris-glycine precast 8% polyacrylamide gels (Novex) so that equal amounts of protein were loaded. Electrophoresis was carried out in 25 mM Tris, 192 mM glycine, and 0.1% SDS (pH 8.3) at 125 V for 1.7 h. The proteins were transferred from the gel to a nitrocellulose membrane (Novex) with a Bio-Rad transfer box at 100 V for 1 h in 25 mM Tris, 192 mM glycine, and 20% methanol (pH = 8.3). The membrane was incubated overnight at 4°C in PBS containing 10% nonfat dried milk and 0.1% Tween 20 to block nonspecific protein binding. To detect the protein of interest (K_V1.2, K_V1.5, or K_V2.1), the nitrocellulose membrane was incubated overnight at 4°C with the primary antibody diluted in PBS containing 0.1% Tween 20 and 1% nonfat dried milk (carrier buffer), followed by incubation for 1 h at room temperature with a horseradish peroxidase-conjugated secondary antibody (Zymed or Jackson Laboratories) diluted in the carrier buffer. The nitrocellulose membrane was washed three times between the first two incubations with the carrier buffer and three times with the carrier buffer plus one time with PBS containing 0.1% Tween 20 after the final incubation. To visualize the antibody, we developed the membranes with enhanced chemiluminescence reagents (ECL, Amersham) and the chemiluminescent signal was captured on X-ray film (ECL Hyperfilm, Kodak). Similar procedures were followed to reprobe the membranes for smooth muscle -actin (Sigma). The bands for each protein were quantified by densitometry.

Statistics. Data are presented as means ± SE. An unpaired t-test or ANOVA with post hoc multiple-comparison test was used to compare data between groups as appropriate. P < 0.05 was considered significant.

Materials. Concentrations for each drug listed in cannulated artery protocols are expressed as final molar concentrations in the vessel bath. ACh, iberiotoxin, and 4-AP were obtained from Sigma. ACh was solubilized in saline, and iberiotoxin was solubilized in H₂O. 4-AP was solubilized in water, and pH was titrated to 7.4 with 12 N HCl. A-23187 and U-46619 were from Biomol and were solubilized with DMSO and EtOH, respectively. Correolide was a generous gift from Merck and Co., Inc. and was solubilized in DMSO. The studies in which correolide was used were performed at Wake Forest University School of Medicine. The K_V1.2 antibody was obtained from Upstate, and the K_V1.5 and K_V2.1 antibodies were from Alomone.

	RESULTS

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
The mean diameter of vessels used for all cannulated artery studies was 210 ± 4 µm for control arteries and 215 ± 5 µm for hypoxic arteries. None of the vehicles used to solubilize the various agents had any effect on arterial diameter.

Transmural pressure and the endothelium do not influence E_m in either artery type. Figure 1 summarizes PASMC E_m determinations for control and hypoxic arteries measured at different transmural pressures. Regardless of transmural pressure, PASMC E_m measurements in hypoxic arteries were less negative (depolarized) compared with control arteries. In addition, for both control and hypoxic arteries, measurements of PASMC E_m were similar for air-infused and intact vessels [for control arteries PASMC E_m was –51 ± 0.4 mV vs. –50 ± 0.8 mV for intact arteries (n = 26 from 9 piglets) and air-infused arteries (n = 9 from 9 piglets), respectively; for hypoxic arteries PASMC E_m was –46 ± 0.5 mV vs. –47 ± 1.4 mV for intact arteries (n = 16 from 9 piglets) and air-infused arteries (n = 6 from 6 piglets)]. Thus neither the presence of the endothelium nor different transmural pressures underlie differences in PASMC E_m between control and hypoxic arteries.

View larger version (19K): [in this window] [in a new window]   Fig. 1. Membrane potential (Em) determinations in 100- to 300-µm-diameter pulmonary arteries of control and hypoxic piglets at transmural pressures of 15 and 25 cmH2O (for control arteries: n = 26 arteries from 9 piglets studied at 15 cmH2O; n = 16 arteries from 9 piglets studied at 25 cmH2O; for hypoxic arteries: n = 9 arteries from 7 piglets studied at 15 cmH2O; n = 16 arteries from 7 piglets studied at 25 cmH2O). All values are means ± SE. *Different from control, 15 cmH2O; #different from control, 25 cmH2O (P < 0.05).

View larger version (14K): [in this window] [in a new window]   Fig. 2. Change in diameter to BaCl2 (10–4 M) or iberiotoxin (10–7 M) for control and hypoxic arteries. For BaCl2, n = 11 arteries from 6 control piglets and n = 7 arteries from 5 hypoxic piglets. For iberiotoxin, n = 7 arteries from 5 control piglets and n = 4 arteries from 4 hypoxic piglets. All values are means ± SE.

View larger version (12K): [in this window] [in a new window]   Fig. 3. A: 4-aminopyridine (4-AP, 10–3 M)-induced changes in Em for arteries from control (n = 10) and hypoxic (n = 5) piglets. All values are means ± SE. *Different from control (P < 0.05). B: 4-AP-induced changes in diameter for endothelium-intact and air-infused arteries from control and hypoxic piglets (n = 19 intact arteries from 15 control piglets; n = 9 air-infused arteries from 8 control piglets; n = 25 intact arteries from 20 hypoxic piglets; n = 7 air-infused arteries from 6 hypoxic piglets). All values are means ± SE. *Different from control intact, #different from control air infused (P < 0.05).

View larger version (9K): [in this window] [in a new window]   Fig. 4. A: correolide-induced changes in diameter for control (n = 13 arteries from 11 piglets) and hypoxic (n = 8 arteries from 8 piglets) arteries. All values are means ± SE. *Different from control (P < 0.05). B: 4-AP (10–3 M)-induced changes in diameter after treatment with correolide (10–6 M) for control (n = 5 arteries from 4 piglets) and hypoxic (n = 5 arteries from 4 piglets) arteries. All values are means ± SE. *Different from control (P < 0.05).

View larger version (21K): [in this window] [in a new window]   Fig. 5. Voltage-gated K+ channel (KV)1.2 -subunit protein in homogenates of 20- to 600-µm-diameter pulmonary arteries from control and hypoxic piglets. Note the lower intensity of bands for the KV1.2 -subunit in homogenates of small pulmonary arteries from hypoxic compared with control piglets. Also note that the intensity of bands for smooth muscle -actin is similar for homogenates from control and hypoxic arteries. In addition, note the lower densitometry units for the KV1.2 bands for hypoxic compared with control arteries. *Different from control (P < 0.05).

View larger version (11K): [in this window] [in a new window]   Fig. 7. KV2.1 -subunit protein in homogenates of 20- to 600-µm-diameter small pulmonary arteries from control and hypoxic piglets. Note the similar intensity of bands for KV2.1 -subunit in homogenates of small pulmonary arteries from control and hypoxic piglets. +, Positive control for KV2.1 -subunits. Also note that there is no difference in the densitometry units between the KV2.1 bands for hypoxic compared with control arteries.

View larger version (12K): [in this window] [in a new window]   Fig. 6. KV1.5 -subunit protein in homogenates of 20- to 600-µm-diameter small pulmonary arteries from control and hypoxic piglets. Note the similar intensity of bands for the KV1.5 -subunit in homogenates of small pulmonary arteries from control and hypoxic piglets. Also note that there is no difference in densitometry units between the KV1.5 bands for hypoxic compared with control arteries.

	DISCUSSION

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

Chronic hypoxia and PASMC E_m. There are limited data regarding the effect of chronic hypoxia on PASMC E_m in newborns. The only other data we are aware of were from freshly isolated PASMC from second-order branches off the intrapulmonary artery of piglets raised in hypoxia for 3 days (11). Consistent with our findings in the intact pressurized artery preparation, E_m in the PASMC were also depolarized (11). Thus, although scarce, the currently available data consistently show that 3 days of chronic in vivo hypoxia alters PASMC membrane properties in small pulmonary arteries of newborns such that E_m is less negative in PASMC of hypoxic piglets than in control piglets.

In comparison to the paucity of data in newborns, the effect of chronic hypoxia on PASMC membrane properties in adult pulmonary arteries has received a lot of attention. It was reported over 20 years ago that PASMC isolated from main pulmonary arteries of adult rats exposed to variable lengths of in vivo hypoxia were depolarized within the first 7 days of hypoxic exposure and remained depolarized for up to 60 days of hypoxic exposure (37). More recent studies have found that after 1–4 wk of in vivo chronic hypoxia PASMC in 200- to 1,200-um-diameter pulmonary arteries and cells isolated from these arteries of adult rats were depolarized (10, 27, 30, 34). Even more recently, it was shown that PASMC isolated from resistance pulmonary arteries exposed to moderate levels of hypoxia for only 24 h were depolarized (15). In addition, PASMC obtained from adult normoxic rats and cultured under hypoxic conditions for 48–72 h were depolarized (25). Thus, with exception of one early report in which PASMC isolated from small pulmonary arteries (200-µm diameter) were hyperpolarized for 15 days and gradually returned to control levels by 40 days of chronic hypoxia (37), the majority of the data clearly show that exposure to chronic hypoxia depolarizes PASMC E_m in both adults and newborns. Moreover, our findings and those of two others (11, 25) indicate that sustained depolarization occurs in PASMC of resistance-level pulmonary arteries after only a few days of in vivo exposure to chronic hypoxia.

K_V channels and newborn PASMC. It is well acknowledged that K⁺ channels are a major determinant of PASMC E_m. Studies with PASMC from adult animals show that of the different K⁺ channels, the K_V channel family plays a significant role in regulation of E_m (43, 44). To evaluate function of the K_V channel family in newborn pulmonary arteries, we used the K_V channel antagonist 4-AP as a pharmacological tool. In normoxic control piglet pulmonary arteries 4-AP elicited constriction and PASMC depolarization. Thus, similar to findings in adults (43, 44), K_V channels in 5- to 7-day-old piglets contribute to regulation of resistance-level pulmonary arterial vasomotor tone and PASMC E_m. Supportive of the notion that K_V channels play a role in regulating tone in the newborn pulmonary circulation, other investigators found that 4-AP elicited vasoconstriction in 700- to 1,200-µm-diameter pulmonary arteries from normoxic newborn piglets either a few hours old or 2 wk old (6). Our results with correolide, a specific blocker of the K_V1 channels, implicate this family in resistance arteries of normoxic newborn piglets. Notably, addition of 4-AP after correolide elicited further constriction, thereby suggesting that although K_V1 channels play a role, other K_V channel families also contribute to the regulation of pulmonary arterial tone in the normoxic newborn piglet. The finding that both iberiotoxin and BaCl₂ elicited constriction suggests that both BK_Ca and K_ir channels are also present and functional in neonatal piglet resistance pulmonary arteries.

Chronic hypoxia and K_V channels in newborn PASMC. K_V channels are regarded as top candidates for the oxygen-sensitive K⁺ channels in PASMC of adult animals (3, 7, 42). It follows that alterations in K_V channels might occur concomitantly with chronic hypoxia-induced changes in PASMC E_m. Indeed, our data from the pulmonary resistance arteries of the hypoxic piglets suggest that K_V channel function is almost completely abolished after 3 days of hypoxia. Findings with correolide indicate impairments in the K_V1 family of channels. In addition, the almost complete lack of arterial constriction to 4-AP after correolide treatment suggests that the function of other K_V channels may also be impaired. Of note, pharmacological blockade of the K_ir and BK_Ca channels in the hypoxic piglets produced constrictions similar to those in arteries from normoxic animals. Thus the function of at least these two other K⁺ channel families remains intact after exposure to 3-day in vivo chronic hypoxia.

Taken together with our immunoblot findings, our data suggest that downregulation of the K_V1.2 channel could underlie, at least in part, the PASMC depolarization and impaired K_V function that occur during exposure to chronic in vivo hypoxia. Alternatively, it must also be considered that sustained depolarization might have downregulated K_V1.2 protein expression as it did expression of K_V1.5 channels in GH3 pituitary cells (16). It should also be considered that our findings indicate that, despite preserved amounts of K_V1.5 and K_V2.1, neither these nor any other K_V channels appear to function after 3-day exposure to chronic hypoxia.

Potential mechanisms involved in chronic hypoxia-mediated inhibition of K_V channel function include elevated cytosolic calcium levels, oxygen radicals, mitochondrial electron chain transport, NADPH oxidase, redox status, metabolic inhibition, cytochrome P-450 oxidoreductase, cytochrome c, cellular redox status changes, endothelin-1 production, conformational changes, and phosphorylation of - and -subunits (9, 19). Which, if any, of these mechanisms underlie altered K_V function in resistance pulmonary arteries of chronically hypoxic newborn piglets remains to be determined. Furthermore, the limited availability of antibodies and more specific pharmacological agents precludes us from evaluating the function and protein expression of all the K_V family channels that might be present and affected by chronic hypoxia in neonatal piglet resistance pulmonary arteries.

Comparing effects of chronic hypoxia on K_V channels in PASMC from adults and newborns. Although we are not aware of any other studies using newborn animals, others have examined the effect of chronic hypoxia on K⁺ channels in the pulmonary circulation of adult animals. Exposure of adult rats to 1–4 wk of in vivo chronic hypoxia augmented the sensitivity to and the magnitude of 4-AP-induced constriction in both first-branch intrapulmonary arteries (10, 22) and 300-µm-diameter pulmonary arteries (27). Isolated, perfused lungs of control rats and rats exposed to hypoxia for 2 days or 3 wk (30) showed similar constrictor responses to 4-AP. Changes in E_m induced by 4-AP were augmented in PASMC isolated from first-branch intrapulmonary arteries of chronically hypoxic rats in one study (22) and did not differ between PASMC from normoxic and chronically hypoxic rats in another study (33). Thus, unlike our findings in pulmonary arteries from newborn piglets, K_V channels in rat pulmonary arteries appear to remain functional with respect to regulation of E_m and vasomotor tone in the pulmonary circulation of hypoxia-exposed adults. It merits comment that although K_V channels appear to remain functional in hypoxic adult rats a number of investigators have shown that K_V channel currents are actually reduced. Neither the length of hypoxia exposure nor whether exposure was in vivo or in vitro appeared to matter. For example, K_V channel currents were decreased in PASMC of adult mice (28) and adult rats exposed to in vivo chronic hypoxia for either 24 h (15) or 2–3 wk (20, 28, 30, 33, 34) and in PASMC of adult rats exposed to 2- to 3-day in vitro chronic hypoxia (25). In contrast, K_V channel activity was unchanged in PASMC from adult humans who had been exposed to hypoxia for 4 wk, but K_Ca activity was attenuated (23). Differences between species, size of arteries used as the source of SMC, and length of hypoxia might account for the disparity in findings between adult humans and rats. Nonetheless, the consistent evidence from studies with rats and mice indicates that chronic hypoxia causes a sustained diminution in K_V current but does not abolish the functional contribution of K_V channels to regulation of E_m or vasomotor tone in the pulmonary circulation of adult animals.

As with newborn piglets, findings with adult models have implicated downregulation of some of the K_V1 channel family members during chronic hypoxia-induced pulmonary hypertension. In vitro studies showed that protein expression of K_V1.2, K_V1.5, and K_V2.1 were decreased in PASMC of adult normoxic rats cultured under hypoxic conditions for 24–72 h (25, 38, 39). In intact animals, protein expression of K_V2.1 and K_V1.5 were decreased in pulmonary arteries isolated from rats exposed to 2–3 wk of chronic in vivo hypoxia (26, 30). A recent, more extensive evaluation of the different K_V channel family subtypes revealed that, in addition to K_V2.1 and K_V1.5, the protein expression of K_V1.1, K_V1.6, and K_V4.3 subunits was also decreased in resistance pulmonary arteries of adult rats exposed to 3 wk of in vivo chronic hypoxia (39). Of note, 3-wk in vivo chronic hypoxia did not alter the protein expression of K_V1.2 subunits in resistance pulmonary arteries of adult rats (39). Thus, whereas we found that 3-day exposure to in vivo chronic hypoxia reduced K_V1.2 but not K_V1.5 or K_V2.1 subunit expression in newborn piglet resistance pulmonary arteries, findings with adult rats suggest that more prolonged, 2- to 3-wk exposure to in vivo hypoxia does not reduce K_V1.2 protein but instead decreases the protein expression of a number of other K_V1 family subunits.

Species differences as well as length of exposure to chronic hypoxia could explain some of the disparity in findings between newborn piglets and adult rats. Segmental and regional diversity in PASMC K⁺ channel distribution should also be considered. Studies with adult pulmonary arteries have shown that proximal segments contain a larger proportion of K_Ca-enriched cells, whereas distal segments contain more K_V-enriched cells (2). In addition, there is evidence for a maturational change in ion channel expression in the pulmonary circulation (31). In sheep the major K⁺ channel regulating E_m in the pulmonary circulation shifts from K_Ca channels in the fetus to K_V channels in the adult (31), and K_V channel expression increases between the newborn period and adulthood (8). Thus it is tempting to speculate that the impaired K_V channel expression and function that we found after 3-day exposure to chronic hypoxia represents an attempt to resume the fetal condition. Further work is needed to more extensively evaluate this possibility. Regardless, it should not be surprising that the influence of chronic hypoxia on specific K⁺ channels varies between newborns and adults.

Limitations of study. Although other types of K⁺ channels, including K_ATP channels (4), may play a role in regulation of pulmonary vascular tone and/or PASMC E_m in newborns, in this study we focused on K_V channels for a number of reasons. First, other investigators have provided evidence that K_ATP channel function is preserved in the pulmonary circulation of newborn piglets exposed to 3 days of chronic hypoxia (4). Second, K_V channels have been implicated in the pathogenesis of pulmonary hypertension in adults (15, 18, 20, 26, 30, 39, 45). Third, evidence from studies with PASMC from adult animals suggests that K_V channels are the O₂-sensitive K⁺ channel (3, 7, 42). We evaluated protein expression of K_V 1.5 and K_V 2.1 because these K_V channel family subunits have been shown to be involved with O₂ sensing in the postnatal pulmonary circulation (3, 40). We also evaluated protein expression of K_V 1.2 because this K_V channel family subunit has been implicated in the pathogenesis of chronic hypoxia-induced pulmonary hypertension in adult animals (25, 38, 39). It is possible that K⁺ channels other than those evaluated in this study are O₂-sensitive K⁺ channels. Moreover, the expression of K_V channel family members other than those we evaluated could be altered in PASMC of newborns exposed to chronic hypoxia. These possibilities merit pursuit as more antibodies and specific pharmacological antagonists become available.

It is important to note that the presence of K_ir channels in PASMC remains uncertain (7, 29, 35). Because it is known that K_ir channels are sensitive to inhibition by extracellular Ba²⁺, our findings that resistance-level pulmonary arteries from control piglets and piglets exposed to 3-day hypoxia constricted to BaCl₂ suggest that these channels are present and functional in PASMC of newborn piglets. However, it is possible that BaCl₂ elicited constriction by mechanisms other than PASMC depolarization via inhibition of K_ir channels. Thus future investigations are needed, including studies utilizing specific antibodies and more specific K_ir pharmacological antagonists and agonists when they become available, to ascertain the presence of and role for K_ir channels in regulating PASMC E_m and pulmonary vascular tone in the normoxic as well as hypoxic pulmonary circulation of both newborns and adults.

Potential impact of altered K_V channel function. Some comments about the potential implications of our findings are warranted. Sustained depolarization such as we found to occur with 3-day exposure to in vivo chronic hypoxia will increase PASMC cytosolic Ca²⁺ (43), which in turn can stimulate PASMC proliferation (24). Furthermore, reduced K_V channel function helps maintain a high concentration of K⁺ in the cytoplasm, which inhibits apoptosis (19). Thus it is possible that sustained PASMC depolarization and concomitant impaired K_V function contribute to the progressive remodeling of the vascular wall that we have shown to occur when hypoxia is extended beyond 3 days (13). It should also be considered that whereas inhibition of K_V channels causes depolarization and constriction, activation of K_V channels leads to hyperpolarization and dilation. Thus the severely impaired function of K_V channels that we found could not only lead to increased basal vascular tone and thereby contribute to the progression of pulmonary hypertension but might have an impact on the effectiveness of dilator therapies used to treat existing pulmonary hypertension.

In summary, our findings show that K_V channels are present and contribute to regulation of E_m and pulmonary vascular tone in newborn piglets that are less than 1 wk old. Exposure to in vivo chronic hypoxia for only a few days depolarizes PASMC, nearly abolishes K_V channel function, and downregulates protein expression of at least one K_V1 channel -subunit, K_V1.2, in resistance pulmonary arteries of newborn piglets. We speculate that development of therapies to counteract these early changes in PASMC properties may help prevent the progressive changes in remodeling and reactivity that occur when hypoxic exposure is extended beyond a few days. Furthermore, that fact that the K⁺ channels responsible for regulation of vasomotor tone might be different in the hypertensive pulmonary circulation should be taken into account when developing therapies to lower pulmonary vascular resistance in infants with pulmonary hypertension associated with chronic hypoxia.

	GRANTS

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
This work was supported by National Heart, Lung, and Blood Institute Grant RO1-HL-68572 (C. D. Fike).

	ACKNOWLEDGMENTS

 
We thank Merck and Co., Inc. for the generous gift of correolide.

	FOOTNOTES

 

Address for reprint requests and other correspondence: C. D. Fike, 2215 B Garland Ave., 1125 MRB IV, Vanderbilt Univ. School of Medicine, Nashville, TN 37232-0656 (e-mail: candice.fike{at}vanderbilt.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. Albarwani S, Nemetz LT, Madden JA, Tobin AA, England SK, Pratt PF, and Rusch NJ. Voltage-gated K⁺ channels in rat small cerebral arteries: molecular identity of the functional channels. J Physiol 551.3: 751–763, 2003.
2. Archer SL, Huang JMC, Reeve HL, Hampl V, Tolarova S, Michelakis E, and Weir EK. Differential distribution of electrophysiologically distinct myocytes in conduit and resistance arteries determines their response to nitric oxide and hypoxia. Circ Res 78: 431–442, 1996.[Abstract/Free Full Text]
3. Archer SL, Souil E, Dinh-Xuan AT, Schremmer B, Mercier JC, Yaagoubi AE, Nguyen-Huu L, Reeve HL, and Hampl V. Molecular identification of the role of voltage-gated K⁺ channels, Kv1.5 and Kv2.1, in hypoxic pulmonary vasoconstriction and control of resting membrane potential in rat pulmonary artery myocytes. J Clin Invest 101: 2319–2330, 1998.[ISI][Medline]
4. Boels PJ, Gao B, Deutsch J, and Haworth SG. ATP-dependent K⁺ channel activation in isolated normal and hypertensive newborn and adult porcine pulmonary vessels. Pediatr Res 42: 317–326, 1997.[ISI][Medline]
5. Cassin S. Role of prostaglandins, thromboxanes, and leukotrienes in the control of the pulmonary circulation in the fetus and newborn. Semin Perinatol 11: 53–63, 1987.[ISI][Medline]
6. Cogolludo A, Moreno L, Lodi F, Tamarag J, and Perez-Vizcaino F. Postnatal maturational shift from PKC and voltage-gated K⁺ channels to RhoA/Rho kinase in pulmonary vasoconstriction. Cardiovasc Res 66: 84–93, 2005.[Abstract/Free Full Text]
7. Coppock EA, Martens JR, and Tamkun MM. Molecular basis of hypoxia-induced pulmonary vasoconstriction: role of voltage-gated K⁺ channels. Am J Physiol Lung Cell Mol Physiol 281: L1–L12, 2001.[Abstract/Free Full Text]
8. Cornfield DN, Saqueton CB, Porter VA, Herron JA, Resnik E, Haddad IY, and Reeve HL. Voltage-gated K⁺ channel activity in ovine pulmonary vasculature is developmentally regulated. Am J Physiol Lung Cell Mol Physiol 278: L1297–L1304, 2000.[Abstract/Free Full Text]
9. Cox RH and Petrou S. Ca²⁺ influx inhibits voltage-dependent and augments Ca²⁺-dependent K⁺ currents in arterial myocytes. Am J Physiol Cell Physiol 277: C51–C63, 1999.[Abstract/Free Full Text]
10. Doggrell SA, Wanstall JC, and Gambino A. Functional effects of 4-aminopyridine (4-AP) on pulmonary and systemic vessels from normoxic control and hypoxic pulmonary hypertensive rats. Naunyn Schmiedebergs Arch Pharmacol 360: 317–323, 1999.[CrossRef][ISI][Medline]
11. Evans AM, Osipenko ON, Haworth SG, and Gurney AM. Resting potentials and potassium currents during development of pulmonary artery smooth muscle cells. Am J Physiol Heart Circ Physiol 275: H887–H899, 1998.[Abstract/Free Full Text]
12. Fike CD and Kaplowitz MR. Chronic hypoxia alters nitric oxide-dependent pulmonary vascular responses in lungs of newborn pigs. J Appl Physiol 81: 2078–2087, 1996.[Abstract/Free Full Text]
13. Fike CD and Kaplowitz MR. Effect of chronic hypoxia on pulmonary vascular pressures in isolated lungs of newborn pigs. J Appl Physiol 77: 2853–2862, 1994.[Abstract/Free Full Text]
14. Fike CD, Pfister SL, Kaplowitz MR, and Madden JA. Cyclooxygenase contracting factors and altered pulmonary vascular responses in chronically hypoxic newborn pigs. J Appl Physiol 92: 67–74, 2002.[Abstract/Free Full Text]
15. Hong Z, Weir EK, Nelson DP, and Olschewski A. Subacute hypoxia decreases voltage-activated potassium channel expression and function in pulmonary artery myocytes. Am J Respir Cell Mol Biol 31: 337–343, 2004.[Abstract/Free Full Text]
16. Levitan ES, Gealy R, Trimmer JS, and Takimoto K. Membrane depolarization inhibits Kv1.5 voltage-gated K⁺ channel gene transcription and protein expression in pituitary cells. J Biol Chem 11: 6036–6041, 1995.
17. Madden JA, Dawson CA, and Harder DR. Hypoxia-induced activation in small isolated pulmonary arteries of the cat. J Appl Physiol 59: 113–118, 1985.[Abstract/Free Full Text]
18. Mandegar M and Yuan J. Role of K⁺ channels in pulmonary hypertension. Vascul Pharmacol 38: 25–33, 2002.[CrossRef][ISI][Medline]
19. Mauban JRH, Remillard CV, and Yuan JXJ. Hypoxic pulmonary vasoconstriction: role of ion channels. J Appl Physiol 98: 415–420, 2005.[Abstract/Free Full Text]
20. Michelakis E and Weir EK. The pathobiology of pulmonary hypertension: smooth muscle cells and ion channels. Clin Chest Med 22: 419–432, 2001.[CrossRef][ISI][Medline]
21. Nelson MT and Quayle JM. Physiological roles and properties of potassium channels in arterial smooth muscle. Am J Physiol Cell Physiol 268: C799–C822, 1995.[Abstract/Free Full Text]
22. Osipenko ON, Alexander D, MacLean MR, and Gurney AM. Influence of chronic hypoxia on the contributions of non-inactivating and delayed rectifier K currents to the resting potential and tone of rat pulmonary artery smooth muscle. Br J Pharmacol 124: 1335–1337, 1998.[CrossRef][ISI][Medline]
23. Peng W, Hoidal JR, Karwande SV, and Farrukh IM. Effect of chronic hypoxia on K⁺ channels: regulation in human pulmonary vascular smooth muscle cells. Am J Physiol Cell Physiol 272: C1271–C1278, 1997.[Abstract/Free Full Text]
24. Platoshyn O, Golovina VA, Bailey CL, Limsuwan A, Krick S, Juhaszova M, Seiden JE, Rubin LJ, and Yuan JXJ. Sustained membrane depolarization and pulmonary artery smooth muscle cell proliferation. Am J Physiol Cell Physiol 279: C1540–C1549, 2000.[Abstract/Free Full Text]
25. Platoshyn O, Yu Y, Golovina VA, McDaniel SS, Krick S, Li L, Wang J-Y, Rubin LJ, and Yuan JX-J. Chronic hypoxia decreases K_V channel expression and function in pulmonary artery myocytes. Am J Physiol Lung Cell Mol Physiol 280: L801–L812, 2001.[Abstract/Free Full Text]
26. Pozeg AI, Michelakis ED, McMurtry MS, Thebaud B, Wu X, Dyck JRB, Hashimoto K, Wang S, Moudgil R, Harray G, Sultanian R, Koshal A, and Archer SA. In vivo gene transfer of the O₂-sensitive potassium channel Kv1.5 reduces pulmonary hypertension and restores hypoxic pulmonary vasoconstriction in chronically hypoxic rats. Circulation 107: 2037–2044, 2003.[Abstract/Free Full Text]
27. Priest RM, Robertson TP, Leach RM, and Ward JPT. Membrane potential-dependent and independent vasodilation in small pulmonary arteries from chronically hypoxic adult rats. J Pharmacol Exp Ther 285: 975–982, 1998.[Abstract/Free Full Text]
28. Raj U and Shimoda L. Oxygen-dependent signaling in pulmonary vascular smooth muscle. Am J Physiol Lung Cell Mol Physiol 283: L671–L677, 2002.[Abstract/Free Full Text]
29. Reeve HL, Archer SL, and Weir EK. Ion channels in the pulmonary vasculature. Pulm Pharmacol Ther 10: 243–252, 1997.[CrossRef][ISI][Medline]
30. Reeve HL, Michelakis E, Nelson DP, Weir EK, and Archer SL. Alterations in a redox oxygen sensing mechanism in chronic hypoxia. J Appl Physiol 90: 2249–2256, 2001.[Abstract/Free Full Text]
31. Reeve HL, Weir EK, Archer SL, and Cornfield DN. A maturational shift in pulmonary K⁺ channels, from Ca²⁺ sensitive to voltage dependent. Am J Physiol Lung Cell Mol Physiol 275: L1019–L1025, 1998.[Abstract/Free Full Text]
32. Shaul PW, Farra MA, and Magness RR. Pulmonary endothelial nitric oxide production is developmentally regulated in the fetus and the newborn. Am J Physiol Heart Circ Physiol 265: H1056–H1063, 1993.[Abstract/Free Full Text]
33. Shimoda LA, Sylvester JT, and Sham JSK. Chronic hypoxia alters effects of endothelin and angiotensin on K currents in pulmonary artery myocytes. Am J Physiol Lung Cell Mol Physiol 277: L431–L439, 1999.[Abstract/Free Full Text]
34. Smirnov SV, Robertson TP, Ward JPT, and Aaronson PI. Chronic hypoxia is associated with reduced delayed rectifier K current in rat pulmonary artery muscle cells. Am J Physiol Heart Circ Physiol 266: H365–H370, 1994.[Abstract/Free Full Text]
35. Snetkov VA, Gurney AM, Ward JPT, and Osipenko ON. Inward rectification of the large conductance potassium channel in smooth muscle cells from rabbit pulmonary artery. Exp Physiol 81: 743–753, 1996.[Abstract]
36. Standen NB and Quayle JM. K⁺ channel modulation in arterial smooth muscle. Acta Physiol Scand 164: 549–557, 1998.[CrossRef][ISI][Medline]
37. Suzuki H and Twarog BM. Membrane properties of smooth muscle cells in pulmonary hypertensive rats. Am J Physiol Heart Circ Physiol 242: H907–H915, 1982.[Abstract/Free Full Text]
38. Wang J, Juhaszova M, Rubin LJ, and Yuan XJ. Hypoxia inhibits gene expression of voltage-gated K⁺ channel alpha subunits in pulmonary artery smooth muscle cells. J Clin Invest 100: 2347–2353, 1997.[ISI][Medline]
39. Wang J, Weigand L, Wang W, Sylvester JT, and Shimoda LA. Chronic hypoxia inhibits K_V channel gene expression in rat distal pulmonary artery. Am J Physiol Lung Cell Mol Physiol 288: L1049–L1058, 2005.[Abstract/Free Full Text]
40. Weir EK, Lopez-Barneo J, Buckler KJ, and Archer SL. Acute oxygen-sensing mechanisms. N Engl J Med 353: 2042–2055, 2005.[Free Full Text]
41. Weir EK, Reeve HL, Huang JMC, Michelakis E, Nelson PD, Hampl V, and Archer SL. Anorexic agents aminorex, fenfluramine, and dexfenfluramine inhibit potassium current in rat pulmonary vascular smooth muscle and cause pulmonary vasoconstriction. Circulation 94: 2216–2220, 1996.[Abstract/Free Full Text]
42. Yuan JXJ. Oxygen-sensitive K⁺ channel(s): where and what? Am J Physiol Lung Cell Mol Physiol 281: L1345–L1349, 2001.[Free Full Text]
43. Yuan JXJ. Voltage-gated K⁺ currents regulate resting membrane potential and [Ca²⁺]_i in pulmonary arterial myocytes. Circ Res 77: 370–378, 1995.[Abstract/Free Full Text]
44. Yuan JXJ, Wang J, Juhaszova M, Golovina VA, and Rubin LJ. Molecular basis and function of voltage-gated K⁺ channels in pulmonary arterial smooth muscle cells. Am J Physiol Lung Cell Mol Physiol 274: L621–L635, 1998.[Abstract/Free Full Text]
45. Yuan XJ, Aldinger A, Juhaszova M, Wang J, Conte JV Jr, Gaine SP, Orens JB, and Rubin LJ. Dysfunctional voltage-gated K⁺ channels in pulmonary artery smooth muscle cells of patients with primary pulmonary hypertension. Circulation 98: 1400–1406, 1998.[Abstract/Free Full Text]
46. Zellers TM and Vanhoutte PM. Endothelium-dependent relaxations of piglet pulmonary arteries augment with maturation. Pediatr Res 30: 176–180, 1991.[ISI][Medline]

This Article Abstract Full Text (PDF) All Versions of this Article: 291/6/L1169    most recent 00117.2006v1 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 ISI Web of Science Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via Google Scholar Google Scholar Articles by Fike, C. D. Articles by Madden, J. A. Search for Related Content PubMed PubMed Citation Articles by Fike, C. D. Articles by Madden, J. A.