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MUSCLE CELL BIOLOGY AND CELL MOTILITY

Myosin light chain kinase activation and calcium sensitization in smooth muscle in vivo

Department of Physiology, University of Texas Southwestern Medical Center, Dallas, Texas

Submitted 21 December 2007 ; accepted in final form 30 May 2008

	ABSTRACT

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Ca²⁺/calmodulin (CaM)-dependent phosphorylation of myosin regulatory light chain (RLC) in smooth muscle by myosin light chain kinase (MLCK) and dephosphorylation by myosin light chain phosphatase (MLCP) are subject to modulatory cascades that influence the sensitivity of RLC phosphorylation and hence contraction to intracellular Ca²⁺ concentration ([Ca²⁺]_i). We designed a CaM-sensor MLCK containing smooth muscle MLCK fused to two fluorescent proteins linked by the MLCK CaM-binding sequence to measure kinase activation in vivo and expressed it specifically in mouse smooth muscle. In phasic bladder muscle, there was greater RLC phosphorylation and force relative to MLCK activation and [Ca²⁺]_i with carbachol (CCh) compared with KCl treatment, consistent with agonist-dependent inhibition of MLCP. The dependence of force on MLCK activity was nonlinear such that at higher concentrations of CCh, force increased with no change in the net 20% activation of MLCK. A significant but smaller amount of MLCK activation was found during the sustained contractile phase. MLCP inhibition may occur through RhoA/Rho-kinase and/or PKC with phosphorylation of myosin phosphatase targeting subunit-1 (MYPT1) and PKC-potentiated phosphatase inhibitor (CPI-17), respectively. CCh treatment, but not KCl, resulted in MYPT1 and CPI-17 phosphorylation. Both Y27632 (Rho-kinase inhibitor) and calphostin C (PKC inhibitor) reduced CCh-dependent force, RLC phosphorylation, and phosphorylation of MYPT1 (Thr694) without changing MLCK activation. Calphostin C, but not Y27632, also reduced CCh-induced phosphorylation of CPI-17. CCh concentration responses showed that phosphorylation of CPI-17 was more sensitive than MYPT1. Thus the onset of agonist-induced contraction in phasic smooth muscle results from the rapid and coordinated activation of MLCK with hierarchical inhibition of MLCP by CPI-17 and MYPT1 phosphorylation.

myosin regulatory light chain; calmodulin; bladder; Rho kinase; myosin light chain phosphatase

The dependence of agonist-induced force and RLC phosphorylation on [Ca²⁺]_i is less than that observed for depolarization in smooth muscle (2, 11) due to Ca²⁺-sensitization mechanisms (33). It is generally assumed, but yet unmeasured, that force is similarly sensitized to MLCK activation. Mechanisms responsible for Ca²⁺ sensitization in smooth muscle involve primarily inhibition of MLCP activity by coupling among ligand receptors, G proteins, and guanine nucleotide-binding factors (33). Two major pathways have been identified for inhibition of MLCP activity in smooth muscle. One involves activation of RhoA and Rho kinase through receptor coupling with mainly G_12/13 heterotrimeric G proteins (35). Rho-kinase phosphorylates myosin phosphatase targeting subunit-1 (MYPT1) at Thr694 and/or Thr850 (mouse sequence), leading to inhibition of MLCP activity in smooth muscle cells and tissues (14, 25, 27, 32, 33). This phosphorylation has been reported to be involved in the tonic phase of force development (6, 39); however, the phosphorylation of both sites is not invariably detectable in all tissues (18, 27). A second pathway involves activation of PKC through receptor coupling with G_q/11 and phospholipase Cβ (17). CPI-17 is a 17-kDa polypeptide and potential mediator of Ca²⁺ sensitization where PKC phosphorylates CPI-17 in smooth muscle (7, 17, 19). Phosphorylation of CPI-17 Thr38 enhances its potency for inhibiting MLCP activity.

To understand how signaling mechanisms involving MLCK activation are integrated with MLCP inhibition in smooth muscle contraction, we developed a genetically encoded sensor for activation of MLCK. The CaM-sensor MLCK contains short smooth muscle MLCK fused to two fluorophores, enhanced cyan fluorescent protein (ECFP) and enhanced yellow fluorescent protein (EYFP), linked by the MLCK calmodulin-binding sequence. Upon dimerization there is significant fluorescence resonance energy transfer (FRET) from the donor ECFP (480 nm emission) to the acceptor EYFP (525 nm emission) (8, 13). This CaM-sensor MLCK is capable of directly monitoring Ca²⁺/CaM binding and activation of the kinase, where Ca²⁺-dependent CaM binding increases kinase activity coincident with a decrease in FRET. The CaM-sensor MLCK is expressed specifically in smooth muscle tissue of transgenic mice to obtain real-time and quantitative information on MLCK activation in vivo in relation to [Ca²⁺]_i, RLC phosphorylation, and isometric force.

We previously reported that membrane depolarization with KCl induced a greater maximal increase in [Ca²⁺]_i and MLCK activation than that obtained with the agonist carbachol (CCh) in bladder smooth muscle from the transgenic mice (13). However, the force development and RLC phosphorylation were comparable. In addition, the Rho-kinase inhibitor Y27632 decreased CCh-induced force while not significantly affecting MLCK activation (13). These results were consistent with the hypothesis that Rho-kinase activation inhibits MLCP to enhance the small extent of agonist-induced MLCK activation. However, the mechanism of this apparent increase in sensitivity to [Ca²⁺]_i with CCh was not fully elucidated. Although some reports showed that MLCP inhibition was induced slowly during tonic contraction in response to agonist treatment (35), MLCP inhibition appeared to occur rapidly during phasic contraction elicited by CCh in the bladder (13). Other evidence also suggests that Rho-kinase modulates contraction in phasic smooth muscle (9, 28, 31, 38). It is proposed for intestinal smooth muscle that there is an initial [Ca²⁺]_i transient leading to MLCK activation and then inactivation followed by MLCP inhibition to sustain RLC phosphorylation and contraction (26). Thus activation of MLCK would be temporally distinct from inhibition of MLCP. In the present study, we test the hypothesis that agonist-induced contraction results from rapid Ca²⁺ sensitization with phosphorylation of CPI-17 and MYPT1 simultaneous with Ca²⁺/CaM-dependent activation of MLCK.

	MATERIALS AND METHODS

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Transgenic mice with CaM-sensor MLCK expression specifically in smooth muscle tissue were bred and screened as previously described (8, 13). Expressed amounts of the MLCK CaM-sensor were <40% the content of endogenous kinase, and stresses generated by bladder strips from wild-type and transgenic animals were comparable (13). Transgenic animals showed no obvious phenotypic differences from wild-type (13). All animal protocols were approved by the University of Texas Southwestern IACUC.

Simultaneous measurement of fluorescence and CaM-sensor MLCK FRET or [Ca²⁺]. Mouse bladder tissues were obtained from 8- to 12-wk-old transgenic mice expressing CaM-sensor MLCK where simultaneous measurements of force and FRET or [Ca²⁺]_i were made as previously described (13). Bladder tissues were dissected into strips (0.5 x 0.5 x 8.0 mm), mounted, and stretched (1.2 x slack length) on a force transducer in a quartz cuvette (180 µl) for simultaneous force and fluorescence measurements in physiological salt solution (PSS, in mM: 118.5 NaCl, 4.74 KCl, 1.18 MgSO₄, 1.18 KH₂PO₄, 24.9 NaHCO₃, 1.6 CaCl₂, and 10.0 D-glucose containing 10 µM indomethacin, pregassed with 95% O₂-5% CO₂ at 36°C). For FRET measurements the muscle strips were illuminated with an excitation wavelength of 430 nm, and emission intensity was measured at both 480 and 525 nm to derive the ratio of fluorescence values (R480/525) in strips contracted with 65 mM KCl (KCl replacing equivalent NaCl in PSS) or 10 µM CCh. After incubation in relaxing solution [in mM: 20 PIPES, 5 magnesium methanesulfonate, 90 potassium methanesulfonate, 4 ATP, 4 EGTA, 1 dithiothreitol, 0.1 diisopropylfluorophosphate; 0.05 trans-epoxysuccinyl-L-leucylamido-(4-guanidino)-butane], muscle strips were skinned with 100 µM β-escin in relaxing solution. The minimum ratio of fluorescence (R_min) was obtained by superfusion with the relaxing solution, whereas the maximum ratio (R_max) and maximum force (F_max) were obtained by adding CaCl₂ to a final concentration of pCa 3.7.

Intracellular calcium concentrations were measured with Indo-1 in intact bladder strips as described previously (13). Urothelium and mucosa layers were removed from intact bladder tissue. Muscle strips were stretched to 1.2 slack length and incubated in the dark with PSS containing 10 µM indo-1 AM, 0.01% pluronic F-127, and 0.02% cremophor for 4 h at room temperature. After being mounted and washed with fresh PSS for 30 min at 36°C, strips were illuminated at 365 nm (D365/10X), and emission intensities were measured at 405 nm (D405/30) and 485 nm (D485/25). The ratio of fluorescence (R405/485) was determined and used to calculate [Ca²⁺]_i. Maximal fluorescence was obtained by superfusion with 50 µM ionomycin in the presence of 5 mM Ca²⁺; minimal fluorescence was obtained with Ca²⁺-free PSS containing 2 mM EGTA. After each experiment, autofluorescence was determined by superfusing with 20 mM Mn²⁺.

Sample preparation. Muscle strips were mounted on isometric force transducers (Grass FT03.C), stretched to 1.2 slack length, and subjected to drug treatments as described. Strips were quick frozen by clamps prechilled in liquid nitrogen after specific treatments for measurements of the extent of phosphorylation of RLC, CPI-17, and MYPT1. Frozen muscles were processed as previously described (13) in 10% trichloroacetic acid followed by centrifugation. The insoluble protein pellets were resuspended in 8 M urea sample buffer containing 18.5 mM Tris (pH 8.6), 20.4 mM glycine, 10 mM dithiothreitol, 4 mM EDTA, 5% sucrose, and 0.004% bromophenol blue and stored at –80°C.

Measurement of RLC and CPI-17 phosphorylation in bladder smooth muscle tissue. Protein samples solubilized in urea sample buffer were subjected to urea-glycerol-PAGE at 400 V for 100 min (RLC) or 150 min (CPI-17) to separate nonphoshorylated and monophosphorylated protein forms. The urea-glycerol-PAGE system separates proteins by mass as well as charge. Phosphorylation results in the addition of two extra negative charges that increases the mobility of the protein during electrophoresis, which is capable of separating nonphosphorylated, monophosphorylated, and diphosphorylated RLC (4, 23). Smooth muscle tissues contain almost exclusively nonphosphorylated and monophosphorylated RLC, in contrast to cells in culture that contain significant amounts of diphosphorylated RLC. Kitazawa and colleagues (19) previously showed for CPI-17 that Thr38 was predominantly phosphorylated by PKC. Thus CPI-17 would be expected to show primarily nonphosphorylated and monophosphorylated forms on urea-glycerol PAGE. If there were additional sites phosphorylated in vivo, distinct diphosphorylated and triphosphorylated proteins would be present.

After electrophoresis, proteins were transferred to polyvinyldifluoride and fixed with 0.4% glutaraldehyde for 30 min. RLC or CPI-17 was visualized by immunoblot using a monoclonal antibody against mouse RLC (generous gift from Kathy Trybus; 21) or a rabbit polyclonal antibody against mouse CPI-17. The polyclonal antibody was raised in rabbits by standard procedures to purified recombinant mouse CPI-17 expressed in Escherichia coli with cDNA kindly provided by Masumi Eto. The antibody binds by Western blot analysis to CPI-17 from mouse, rabbit, pig, and rat (data not shown). The ratio of phosphorylated RLC or CPI-17 to total (nonphosphorylated and monophosphorylated) was determined by quantitative densitometry and expressed as moles of phosphate per moles of protein.

Measurement of MYPT1 phosphorylation. Protein samples prepared in urea sample buffer were added to 0.2 volume of SDS sample buffer containing 250 mM Tris (pH 6.8), 10% SDS, 50 mM dithiothreitol, 40% glycerol, and 0.01% bromophenol blue, and then boiled and subjected to SDS-PAGE. Proteins were transferred to nitrocellulose and visualized by immunoblot using antibodies to either total MYPT1 or phospho-MYPT1 at Thr694 or Thr850 (mouse sequence) (Upstate, Waltham, MA). The phosphorylation of MYPT1 is expressed as the ratio relative to that obtained with tissues treated for 1 min with 10 µM CCh in the presence of 5 µM okadaic acid (a protein phosphatase type 1 and type 2a inhibitor).

Statistics. Statistical comparisons were performed by paired Student's t-test for [Ca²⁺]_i and MLCK activation, independent t-test for force development, and phosphorylation of RLC, CPI-17, and MYPT1. Two-tailed values were used and P values <0.05 were considered significant.

	RESULTS

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Time course of responses to depolarization and agonist. Both KCl and CCh elicit transient force development in the phasic bladder smooth muscle. Bladder strips were stimulated for 1 or 5 min with KCl (65 mM) or CCh (10 µM) and force, RLC phosphorylation, intracellular calcium, and MLCK activation were measured (Fig. 1). Rates of force development were similar for KCl and CCh with times to peak of 41 ± 5 s and 31 ± 7 s, respectively; forces at 1 min were near maximal at 87 ± 6% and 87 ± 3% (n = 8, 7), respectively. Agonist-dependent sensitization of force to [Ca²⁺]_i and MLCK activation was well manifested at 1 min of stimulation where forces comparable to KCl were obtained by CCh at one-half the value of MLCK activation (Fig. 1). At 5 min of stimulation, force was reduced to low but significantly elevated values following reductions in [Ca²⁺]_i and MLCK activation (Fig. 1). However, both [Ca²⁺]_i and MLCK activation remained significantly elevated above resting values at 5 min. Agonist-dependent sensitization of force was also observed at 5 min where comparable forces were achieved with CCh compared with KCl at about one-half the value of MLCK activation.

View larger version (17K): [in this window] [in a new window]   Fig. 1. Time course of responses to KCl and carbachol (CCh). Bladder strips were stimulated by 65 mM KCl for 1 or 5 min (KCl 1, KCl 5) or by 10 µM CCh for 1 or 5 min (CCh 1, CCh 5). Intracellular Ca2+ concentration ([Ca2+]i), myosin light chain kinase (MLCK) activation (A), regulatory light chain (RLC) phosphorylation, and force (B) were plotted. Values are means ± SE; n = 5–7 animals. *P < 0.05 when compared with value at rest; #P < 0.05 when compared with same treatment at 1 min.

View larger version (9K): [in this window] [in a new window]   Fig. 2. Dependence of force on MLCK activation and RLC phosphorylation in bladder smooth muscle stimulated by KCl or CCh. A: MLCK activation and force were measured in bladder muscle strips from transgenic mice stimulated with 30, 40, 50, and 65 mM KCl (, n = 5) or with 0.3, 1, 3, 10, and 30 µM CCh (, n = 8). Measurements were obtained at 1 min. Contraction was normalized by the 65 mM KCl-induced contraction for each strip. B: force was measured in bladder muscle strips stimulated with concentrations of KCl (, n = 5) or CCh (, n = 5) as described in A. Strips were frozen at 1 min and processed for measurement of RLC phosphorylation. Values are means ± SE.

View larger version (18K): [in this window] [in a new window]   Fig. 3. Phosphorylation of PKC-potentiated phosphatase inhibitor (CPI-17) and myosin phosphatase targeting subunit-1 (MYPT1) in bladder strips in response to 65 mM KCl or 10 µM CCh. A: Western blot analysis of tissue extracts subjected to urea-glycerol PAGE and detected with anti-CPI-17 antibody. Top band, nonphosphorylated CPI-17; bottom band, phosphorylated CPI-17. B: Western blot analysis of tissue extracts subjected to SDS PAGE and detected with anti-MYPT1 or anti-phospho-MYPT1 (Thr694) antibodies. C: phosphorylation of CPI-17 with KCl treatment at 1 and 5 min (KCl 1, KCl 5) or CCh treatment at 1 and 5 min (CCh 1, CCh 5), (n = 10–13). Ratio of phosphorylated CPI-17 to total (unphosphorylated and phosphorylated) is expressed as moles of phosphate per mole of protein. D: phosphorylation of MYPT1 with KCl or CCh treatment for times as indicated in C (n = 7–9). Phosphorylation of MYPT1 is expressed as the ratio relative to that stimulated with CCh in the presence of 5 µM okadaic acid (OA). Values are means ± SE. *P < 0.05 when compared with value at rest; #P < 0.05 when compared with same treatment at 1 min.

View larger version (16K): [in this window] [in a new window]   Fig. 4. Effects of Y27632 or calphostin C on CCh-induced responses of bladder strips. [Ca2+]i and MLCK activation (n = 7) (A) and RLC phosphorylation and force (n = 5–7) (B) are plotted. Strips were preincubated 15 min with 10 µM Y27632 (Y+CCh) or 1 µM calphostin C (C+CCh) followed by 1 min with 10 µM CCh (CCh) as indicated. Values are means ± SE; n = 14. *P < 0.05 when compared with value at rest; #P < 0.05 when compared with CCh alone.

View larger version (12K): [in this window] [in a new window]   Fig. 5. Effects of Y27632 and calphostin C on phosphorylation of CPI-17 and MYPT1 in bladder strips in response to CCh. Strips were preincubated for 15 min with 10 µM Y27632 (Y+CCh) or 1 µM calphostin C (C+CCh) followed by 1 min with 10 µM CCh as indicated. Phosphorylations of CPI-17 (A) and MYPT1 (Thr694) (B) were assessed as described in Fig. 3. Values are means ± SE; n = 7–9. *P < 0.05 when compared with value at rest; #P < 0.05 when compared with CCh alone.

View larger version (10K): [in this window] [in a new window]   Fig. 6. Dependence of CPI-17 and MYPT1 phosphorylation on CCh concentration. Strips were incubated 1 min at indicated concentrations. The percent change in phosphorylation of CPI-17 () or MYPT1 (Thr694) () was calculated as the difference between resting and stimulated values and normalized by the maximal change observed. CPI-17 and MYPT1 phosphorylation values were determined as described in Fig. 3. Values are means ± SE; n = 5–7.

	DISCUSSION

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION GRANTS REFERENCES

Agonist-induced Ca²⁺ sensitization in smooth muscle is known to result from inhibition of MLCP activity primarily through signaling pathways that target CPI-17 and/or MYPT1 for phosphorylation (33). In this study, the Rho-kinase inhibitor Y27632 and PKC inhibitor calphostin C diminished RLC phosphorylation and force development without affecting MLCK activation, indicating that agonist-induced RLC phosphorylation and force result from not only MLCK activation but also involve Rho kinase and PKC activation. Elevated phosphorylation of MYPT1 and CPI-17 with CCh at 1 min supports the hypothesis that MLCP activity is inhibited by both MYPT1 and CPI-17 phosphorylation. CPI-17 phosphorylation was attenuated by calphostin C but not by Y27632, which is consistent with PKC-mediated phosphorylation. Interestingly, calphostin C did not reduce CPI-17 phosphorylation below that found in resting muscle, which was a significant amount (0.25 mol/mol). It has been reported that protein kinases other than PKC can phosphorylate CPI-17 in vitro: ZIP-like kinase (22), protein kinase N (10), integrin-linked kinase (5), p21-activated kinase (40), and Rho kinase (20). However, Y27632 had no effect on CPI-17 phosphorylation, suggesting that the transient phosphorylation induced by CCh and the extent of phosphorylation in resting muscle do not result from Rho-kinase activity. Furthermore, although CPI-17 phosphorylation occurred rapidly, it was not sustained. Thus CPI-17 phosphorylation would not be involved in Ca²⁺ sensitization during the latter phase of the contraction.

In contrast, MYPT1 phosphorylation at the inhibitory site Thr694 induced by CCh treatment was abolished by both calphostin C and Y27632, which were associated with attenuation of RLC phosphorylation and force. These results support a role for MYPT1 phosphorylation in inhibiting MLCP activity, although the calphostin C results are difficult to interpret mechanistically because PKC has not been reported to directly phosphorylate MYPT1. Our results with the bladder are consistent with those in another phasic smooth muscle, the ileum, where PKC inhibitors diminished MYPT1 phosphorylation (12). It is possible that PKC may affect some upstream signaling target that leads to MYPT1 phosphorylation by either Rho kinase or integrin-linked kinase (12). Recent studies reported direct or indirect interactions of PKC with RhoA in different cell types (1, 28, 30, 32), although the exact mechanism by which Rho kinase is activated by PKC remains elusive. It is possible that the decrease of MYPT1 phosphorylation by calphostin C results in part from inhibition of RhoA/Rho-kinase pathway via PKC activation.

The phosphorylation site of MYPT1 in smooth muscle stimulated with agonist needs to be considered. There are two major phosphorylation sites on MYPT1, Thr694 and Thr850, and several minor sites mediated by Rho-kinase activation (33). Thr694 phosphorylation by Rho kinase has been detected in a variety of cells including smooth muscle (14, 36, 38), and this phosphorylation is inhibited by Y27632. Previous studies show a positive correlation between Thr694 phosphorylation and force in smooth muscle tissue with agonist treatment (14, 29, 32). However, it is not invariably detectable in intact tissues showing Ca²⁺ sensitization (18, 27, 42). The reasons for this inconsistency are not clear. They may depend partly on the type of cells/tissues, methods of stimulation, or developmental regulation of MYPT1 (3). Additional analysis of data in different types of smooth muscle tissue stimulated with agonists that activate different signaling pathways may provide insights.

Depolarization by KCl did not lead to changes in phosphorylation of either Thr694 on MYPT1 or CPI-17 in the mouse bladder. However, KCl-dependent phosphorylation of MYPT1 or CPI-17 has been observed in vascular smooth muscle (6, 41). Preliminary data with the bladder indicate that, like Thr694, phosphorylation of Thr850 on MYPT1 was not changed with KCl treatment (0.25 ± 0.03 and 0.31 ± 0.05, control and stimulated 1 min, respectively). The dependence of force on MLCK activation with KCl is not entirely linear (Fig. 2A), suggesting that sensitization may occur at higher concentrations. Unlike the case for CCh, this effect does not appear to arise from inhibition of myosin phosphatase activity as neither MYPT1 nor CPI-17 phosphorylations are affected, and force is significantly elevated with no change in RLC phosphorylation between 50 and 65 mM KCl (Fig. 2B). Whereas this observation is tangential to the present study, it warrants speculation as to whether the effect reveals minor forms of regulation possibly mediated through actin-binding proteins caldesmon or calponin, though the physiological importance of thin filament regulation remains unclear (33). It is also worth noting a second aspect of the phasic contraction in mouse bladder, which is the apparent desensitization of contraction to calcium, as defined by the greater reduction in force than [Ca²⁺]_i between 1 and 5 min, particularly evident with KCl. This phenomenon has been observed in skinned fibers of phasic smooth muscles as well and is shown to be calcium dependent, although the mechanism remains to be defined (24).

It is evident that the relative contributions of CPI-17 and MYPT1 in regulating MLCP activity differ depending on the time, type, and intensity of stimulation for a specific smooth muscle. In this study of phasic urinary bladder muscle, results suggest that both CPI-17 and MYPT1 participate in the early phase of sensitization, whereas only MYPT1 participates in the latter phase. This contrasts with tonic muscle, where only CPI-17 is phosphorylated in the early phase, and both CPI-17 and MYPT1 are phosphorylated in the sustained phase of contraction (6). Tonic, compared with phasic, smooth muscle contains relatively high ratios of CPI-17 to MYPT1, shows greater potentiation in response to activators of PKC, and thus utilizes CPI-17 extensively in regulating contraction (5, 43). Whereas phasic muscles may rely less on signaling to CPI-17, classification by tissue origin in rabbit revealed a gradation in PKC-dependent calcium sensitization where airway>bladder>vas deferens, with bladder using this pathway for nearly half the total response (43). We found at low agonist concentrations, only CPI-17 was phosphorylated, with MYPT1 phosphorylation recruited as CCh concentration was raised to higher values (Fig. 6). This may suggest that muscarinic receptors in the bladder signal more effectively through the G_q/11-phospholipase Cβ pathway than through the G_12/13-RhoGEF pathway to inhibit myosin phosphatase. It is interesting to speculate that the accelerated sensitization seen at high CCh concentrations (Fig. 2) may result from the recruitment of phospho-MYPT1. The respective contributions of CPI-17 and MYPT1 to Ca²⁺ sensitization will depend on their expression levels as well as extents of phosphorylation, which varies in different types of smooth muscle tissues.

In conclusion, our genetically encoded CaM-sensor MLCK provides opportunities for investigations on physiological processes involved in smooth muscle contraction. Results from these studies in bladder smooth muscle suggest that agonist-induced contraction results from the rapid and coordinated activation of Ca²⁺/CaM-dependent MLCK that is significantly sustained as well as inhibition of MLCP through phosphorylation of CPI-17 and MYPT1.

	GRANTS

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This study was supported by a grant from the National Heart, Lung, Blood Institute (HL-26043), the Moss Heart Fund, and the Fouad A. and Val Imm Bashour Distinguished Chair in Physiology (to J. T. Stull).

	DISCLOSURES

 
Current address of E. Isotani: Dept. of Neurosurgery, Tokyo Medical and Dental University, 1-5-45 Yushima, Bunkyoku, Tokyo, 113-8519.

	FOOTNOTES

 

Address for reprint requests and other correspondence: K. E. Kamm, Dept. Physiology, UT Southwestern Medical Center, 5323 Harry Hines Blvd., Dallas, TX 75390-9040 (e-mail: kristine.kamm{at}utsouthwestern.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.

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