These authors contributed equally to this work;
Germinal center-specific protein human germinal center associated lymphoma directly interacts with both myosin and actin and increases the binding of myosin to actin
Article first published online: 20 APR 2011
© 2011 The Authors Journal compilation © 2011 FEBS
Volume 278, Issue 11, pages 1922–1931, June 2011
How to Cite
Lu, X., Kazmierczak, K., Jiang, X., Jones, M., Watt, J., Helfman, D. M., Moore, J. R., Szczesna-Cordary, D. and Lossos, I. S. (2011), Germinal center-specific protein human germinal center associated lymphoma directly interacts with both myosin and actin and increases the binding of myosin to actin. FEBS Journal, 278: 1922–1931. doi: 10.1111/j.1742-4658.2011.08109.x
- Issue published online: 17 MAY 2011
- Article first published online: 20 APR 2011
- Accepted manuscript online: 29 MAR 2011 10:52PM EST
- (Received 2 February 2011, revised 21 March 2011, accepted 24 March 2011)
- germinal center;
Human germinal center associated lymphoma (HGAL) is a germinal center-specific gene whose expression correlates with a favorable prognosis in patients with diffuse large B-cell and classic Hodgkin lymphomas. HGAL is involved in negative regulation of lymphocyte motility. The movement of lymphocytes is directly driven by actin polymerization and actin–myosin interactions. We demonstrate that HGAL interacts directly and independently with both actin and myosin and delineate the HGAL and myosin domains responsible for the interaction. Furthermore, we show that HGAL increases the binding of myosin to F-actin and inhibits the ability of myosin to translocate actin by reducing the maximal velocity of myosin head/actin movement. No effects of HGAL on actomyosin ATPase activity and the rate of actin polymerization from G-actin to F-actin were observed. These findings reveal a new mechanism underlying the inhibitory effects of germinal center-specific HGAL protein on lymphocyte and lymphoma cell motility.
diffuse large B-cell lymphoma
human germinal center associated lymphoma
RhoA-specific guanine nucleotide exchange factor
Lymphocyte migration to inflammatory sites and into and out of lymphoid organs is essential for organizing secondary immune anatomical structures such as lymphoid follicles and germinal centers (GC), permitting the appropriate development and propagation of immune responses. In GC, B-cell responses to antigens are amplified and refined in specificity . GC B-lymphocytes are functionally and spatially segregated from extra-GC compartments as a result of limited inter-compartmental lymphocyte movement [2–6]. Although restriction to the GC compartment may be necessary for successful completion of the GC reaction, the molecular mechanisms decreasing GC B-cell motility and GC exit are largely unknown.
We have recently cloned the gene for HGAL that is specifically expressed in GC B-lymphocytes . HGAL is also expressed in GC-derived lymphomas and identifies biologically distinct subgroups of diffuse large B-cell lymphomas (DLBCL), as well as classic Hodgkin lymphoma associated with improved survivals [7–10]. Studies of HGAL murine homolog encoding the M17 protein using M17 knockout mice revealed that this protein is dispensable for GC formation, immunoglobulin somatic hypermutation and class-switch recombination, as well as mounting of T cell-dependent antibody responses . However, M17-deficient mice exhibited reduced-sized Peyer’s patches . We reported that HGAL inhibits the migration of GC B-cells and HGAL-expressing lymphoma cells by activating the RhoA signaling pathway . The effect of HGAL on RhoA is mediated by its direct interaction with RhoA-specific guanine nucleotide exchange factors (RhoGEFs), PDZ-RhoGEF and LARG, that stimulate the GDP-GTP exchange rate. Although this effect may underlie the inhibitory effects of HGAL on the motility of GC lymphocyte and GC-derived lymphoma cells, we also observed that HGAL coimmunoprecipitates and colocalizes with actin and myosin proteins , suggesting that additional molecular mechanisms may contribute to the inhibitory effect of HGAL on B-cell motility. In the present study, we demonstrate that HGAL protein can directly and independently bind to both cellular actin and myosin II proteins. We have also identified the regions within HGAL and myosin that mediate the interaction between HGAL and myosin II. Furthermore, we demonstrate that HGAL increases the binding of myosin to filamentous actin (F-actin) and inhibits the ability of myosin to translocate F-actin. These molecular mechanisms may further contribute to the inhibitory effects of HGAL on the motility of GC lymphocyte and GC-derived lymphoma cells.
HGAL protein directly interacts with both F-actin and myosin
Using a co-immunoprecipitation assay and colocalization studies, we have previously shown that HGAL protein interacts with both actin and myosin II . To determine whether the interaction is direct or indirect, we conducted actin-HGAL and myosin–HGAL cosedimentation assays using purified recombinant HGAL and purified nonmuscle F-actin and rabbit skeletal muscle myosin II proteins. As shown in Fig. 1A, after centrifugation, the majority of the HGAL protein was pulled down into the pellets with F-actin. Similarly, as indicated in Fig. 1B, almost all of the HGAL protein was precipitated with myosin. The binding of HGAL to F-actin and myosin was saturable and occurred at molar ratios of 5 : 1 and 2.5 : 1, respectively. The results obtained show that HGAL co-precipitates with both actin and myosin, suggesting that the interactions between HGAL and both actin and myosin are direct and independent.
HGAL binds to the head and tail regions of myosin
Because we have demonstrated a direct and independent binding of HGAL to myosin, we next carried out experiments aiming to identify the domains of myosin where HGAL binds, as well as the region of HGAL that interacts with myosin. We constructed plasmids that express the N-terminal portion of HGAL protein (pcDNA3.1V5 HGAL delta C encoding amino acids 1–118 of the HGAL protein) and plasmids that express the head region of myosin (subfragment 1 or S1), as well as the rod and tail regions. The myosin proteins pEGFP myosin (1–843) (the head region), pEGFP myosin (844–1665) (the rod region) and pEGFP myosin (1666–1961) (the tail region) can be expressed in 293Tcells (Fig. 2A). Co-immunoprecipitation experiments demonstrated that HGAL interacts with the myosin head (S1) and tail regions but not with the rod region (Fig. 2B,C). A search for potential HGAL consensus binding motif in the myosin head (S1) and tail regions failed to identify identical 5–8 amino acid sequences in these regions, suggesting that binding to different motifs occurs. HGAL does not interact with the myosin light chains (data not shown). We further demonstrate that the N-terminal portion of the HGAL (amino acids 1–118) is sufficient to allow its interaction with myosin (Fig. 2C). Overall, these studies demonstrate that the N-terminal portion of the HGAL protein (amino acids 1–118) can bind to the tail and head (S1) regions of myosin II, with the latter containing the actin and ATP binding sites, but does not bind to the rod part of the myosin molecule that is responsible for filament formation.
HGAL increases binding of myosin to F-actin
HGAL is involved in the negative regulation of lymphocyte migration . Cell movement appears to be driven directly by actin polymerization and by actin–myosin interactions. The effect of HGAL on the binding of myosin to F-actin was examined using a fluorescence-based assay and pyrene labeled F-actin. As shown in Fig. 3, the binding of myosin to F-actin was 54-fold stronger in the presence of HGAL compared to the absence of HGAL. The respective Kd values (in nm) were Kd = 10.8 ± 2.6 (n = 11 independent experiments) in the absence of HGAL and Kd = 0.2 ± 0.5 in the presence of HGAL (n = 10). The difference was statistically significant (P < 0.01). Thus, HGAL can increase the interaction between myosin II and F-actin. A negative control experiment showed no effect of BSA on binding of myosin to F-actin (data not shown), suggesting a specific HGAL-mediated effect on Kd.
HGAL inhibits the ability of myosin to translocate actin
To determine whether HGAL affects the interaction between myosin and actin at the molecular level, we measured the ability of myosin to translocate actin filaments in an in vitro motility assay . Unloaded actin filament velocity was measured over a range of myosin concentrations in the presence and absence of HGAL. Figure 4 shows that actin filament velocity was relatively insensitive to myosin concentrations over a broad range (100–400 μg·mL−1) both in the presence and absence of HGAL. However, the velocity at which saturation occurred (Vsat) was reduced in the presence of HGAL (P = 0.05).
At myosin loading concentrations below the point of Vsat (< 100 μg·mL−1), the number of filaments moving on the surface was reduced and the average velocity was decreased. Actin filaments will move at maximum velocity in the motility assay when surface concentrations are sufficient to allow at least one myosin head to interact with the moving filament at all times. At concentrations below Vsat, the velocity slows because there are prolonged periods of time where there are no myosin molecules bound to and moving the actin filament. Thus, the amount of myosin required to achieve maximal velocity gives a qualitative determination of the duty cycle (i.e. the fraction of myosin ATPase cycle where myosin is strongly bound to actin). The data show that actin filament velocity reaches maximum velocity at a similar myosin concentration in the presence and absence of HGAL. Therefore, although HGAL inhibits maximal velocity, the unloaded duty cycle of the isolated actomyosin is unaffected.
HGAL has no effect on actomyosin ATPase activity and actin polymerization
Actin polymerization and the actomyosin ATPase activity are required for chemotaxis and cytokinesis. Therefore, we hypothesized that HGAL may affect actin polymerization and/or the actomyosin ATPase activity. As shown in Fig. 5, the actin activated myosin ATPase activity was not affected by HGAL and no significant differences in the activity levels were observed in the presence of HGAL. Similarly, no effect of HGAL on the rate of actin polymerization was observed (Fig. 6).
Lymphocyte motility and migration are critical features of various physiological and pathological processes, including immune response and lymphoma dissemination. Lymphocyte motility is a multistep process that results from a coordinated cytoskeletal remodeling primarily mediated by cyclic interactions between the myosin head domains projecting from the myosin filaments and polymerized F-actin in the presence of ATP. Hydrolysis of the ATP by myosin releases free energy that is utilized to generate a mechanical force for directed actin-based movement. In the case of skeletal muscle, this complex process is regulated by the tropomyosin–troponin regulatory proteins that control the actin–myosin interaction depending on calcium ion concentrations in the cell. In nonmuscle cells, other distinct proteins may control actin–myosin interaction.
The regulatory processes controlling lymphocytes motility, especially the motility of GC lymphocytes and lymphoma cells, are not fully elucidated. In the GC, B-lymphocytes are functionally and spatially segregated from extra-GC compartments. Some of the GC B-lymphocytes demonstrate restricted motility between the light and dark zones of the GC , whereas other B cells are stationary throughout these zones. Additionally, in contrast to largely spherical naïve and memory B lymphocytes, GC B-cells frequently exhibit irregular contours with shifting prominent cytoplasmic processes, resulting in polarized shapes [2–5]. These observations may suggest the existence of GC B-cell unique cytoskeletal regulatory proteins. Indeed, HGAL (also named germinal center-expressed transcript 2-GCET2) is specifically expressed in GC B-lymphocytes and GC-derived lymphomas and decreases lymphocyte motility [9,12,13]. We have demonstrated that the inhibitory effect of HGAL on lymphocyte motility may partly be attributed to the activation of the RhoA signaling pathway . The effect of HGAL effect on RhoA is mediated by its direct interaction with the RhoGEFs, PDZ-RhoGEF and LARG, that stimulate the GDP–GTP exchange rate and the activation of RhoA downstream effectors that regulate cytoskeletal remodeling. However, as shown by co-immunoprecipitation experiments , we previously found that HGAL colocalizes and interacts with actin and myosin II, suggesting additional mechanisms that may contribute to the inhibitory effect of HGAL on cell motility. In the present study, by using recombinant purified HGAL and purified F-actin and myosin proteins in cosedimentation assays, we demonstrate that HGAL interacts directly and independently with both actin and myosin. These findings corroborate our previous observations that inhibiting actin polymerization and disrupting microfilament organization with cytochalasin D or latrunculin B did not affect HGAL-myosin interactions . We show that the N-terminal portion of the HGAL protein can interact with two myosin regions, namely the head (S1) and tail, but not with the rod region. Although the tail domain generally mediates interaction with the ‘cargo’ and/or other myosin molecules, the head domain is involved in binding to F-actin, which is coupled to steps in the hydrolysis of ATP and the transduction of free energy into directed actin-based movement. As demonstrated in the present study, HGAL does not affect the actomyosin ATPase activity, although it significantly increases the strength of actin-myosin binding. This may lead to prolongation of the myosin–actin interaction and contribute to a decreased ability of myosin to translocate actin. An HGAL-induced decrease in actin filament sliding velocity, as shown by the in vitro motility assays, supports this idea. Alternatively, but not mutually exclusive, HGAL binding to myosin and/or actin may serve as a ‘load’ that resists actin filament motion, thus leading to the same effects. It can be hypothesized that HGAL functions as a molecular tether between the thick myosin-containing filaments and filamentous actin, and regulates the kinetics of acto–myosin interactions and thus cellular motility. The HGAL-mediated bridging properties are similar to those imposed by another myosin binding protein, myosin-binding protein C, which is shown to form a linkage between the thick and thin filaments of cardiac muscle and regulate cardiac contractility [15,16]. Similar to HGAL, myosin-binding protein C can bind to two different regions in the myosin molecule and affect actomyosin motility . The finding of no change in actomyosin ATPase activity suggests that HGAL does not affect the number or rate of myosin cross-bridges undergoing a transition from the weakly to strongly bound state and the generation of force. Overall, these findings demonstrate that HGAL interaction with actin and myosin may contribute to the decreased motility of GC lymphocytes expressing HGAL protein.
Previous studies in mice identified regulators of actin dynamics and cell motility as key determinants of in vivo lymphoma progression . Specifically, inhibition of cytoskeletal remodeling resulted in decreased lymphoma dissemination and progression. HGAL expression in human DLBCL tumors was associated with limited stage and prolonged survival [7,19]. HGAL regulation of actin dynamics via RhoA activation and the direct effects on actin–myosin interactions may explain the association between HGAL expression and the favorable outcome of DLBCL and classical HL patients whose tumors express this protein, which is consistent with observations in mice. Because HGAL is specifically expressed only in GC lymphocytes and GC-derived lymphomas, further studies are needed aiming to investigate the unique role of HGAL-mediated inhibition of lymphocyte motility on immune response and in lymphomagenesis.
Furthermore, it is of note that both RhoA GTPase and actin cytoskeleton have been implicated in B-cell receptor (BCR) signaling. Saci et al.  showed that RhoA is activated in response to BCR stimulation and affects BCR-dependent calcium flux and cell proliferation. In addition, it was demonstrated that BCR stimulation induces rapid global actin depolymerization in a BCR signal strength-dependent manner followed by polarized actin repolymerization and actin depolymerization enhanced BCR signaling . Because HGAL can regulate the activation of RhoA and affects actomyosin cytoskeleton, it is possible that HGAL may also contribute to the regulation of the BCR signaling. These studies are currently ongoing in our laboratory.
Cells, cell culture, plasmids and transfection
HEK 293 cells were cultured at 37 °C and 5% CO2 in DMEM (Mediatech, Manassas, VA, USA), supplemented with 10% fetal bovine serum (Hyclone, Logan, UT, USA), 2 mm glutamine and 100 units·mL−1 penicillin and 100 μg·mL−1 streptomycin (Invitrogen-Gibco, Grand Island, NY, USA).
The full length wild-type human nonmuscle myosin IIA heavy chain plasmid pEGFP-myosin IIA and its truncated mutant pEGFP-myosin II ARF (1666–1961) [22,23] were generous gifts from Dr Masayuki Takahashi (Division of Chemistry, Graduate School of Science, Hokkaido University, Sapporo, Japan). Using standard cloning techniques, truncated mutants encoding the head portion of myosin IIA linked to EGFP (pEGFP1-843) and the rod part of myosin IIA linked to EGFP (pEGFP844–1665) were generated from the pEGFP-myosin IIA plasmid that was used as a template. The vectors pcDNA3.1V5HGAL and pcDNA3.1V5 HGAL delta C encoding amino acids 1–118 of the HGAL protein have been reported previously .
Polyfect transfection reagent (Qiagen, Valencia, CA, USA) was used for the transfection of plasmids into HEK 293 cells in accordance with the manufacturer’s instructions. Briefly, cells were plated at 2 × 106 cells in 100-mm culture dishes (Nalge Nunc International, Rochester, NY, USA) in 10 mL of DMEM and grown overnight at 37 °C and 5% CO2. Plasmid DNA (8 μg), diluted and mixed in 300 μL of serum-free DMEM was incubated for 5 min at room temperature. Polyfect transfection reagent was added to the mixture, which was incubated for an additional 10 min at room temperature and then added to the cells in a dropwise manner. The cells were incubated for 48 h before proceeding with the subsequent experiments.
Antibodies, western blot analysis and immunoprecipitation
Mouse monoclonal HGAL antibody was generated in our laboratory, as described previously . Mouse monoclonal GFP antibody was obtained from Santa Cruz Biotechnology Inc. (Santa Cruz, CA, USA) and mouse monoclonal V5 antibody was obtained from Invitrogen Inc. (Carlsbad, CA, USA). Western blotting and immunoprecipitation were performed as described previously . Briefly, whole-cell extracts were prepared by lysing 5 × 106 cells in radioimmunoprecipitation assay buffer (1× phosphate-buffered saline, 1% Nonidet P-40, 0.5% sodium deoxycholate, 0.1% SDS, 10 mm phenylmethanesulfonyl fluoride, 1 μg·mL−1 aprotinin, 100 mm sodium orthovanadate) on ice for 30 min. Cell lysate was centrifuged at 14 000 g for 10 min at 4 °C. Protein concentration of lysates was determined using Coomassie protein assay reagent (Thermo Scientific, Rockford, IL, USA) and samples were adjusted to an equal protein concentration. For immunoprecipitation, 400 μg of protein was precipitated for 1–2 h with the indicated antibody at 4 °C with rotation. Protein G-agarose (Invitrogen) or TrueBlotTM anti-Mouse Ig Immunoprecipitation Beads (eBioscience, Carlsbad, CA, USA) were added and the mixture was rotated for a 1 h. Precipitated complexes were washed four times in radioimmunoprecipitation assay buffer, boiled in Laemmli buffer (2× concentrate: 4% SDS, 20% glycerol, 10% 2-mercaptoethanol, 0.004% bromophenol blue, 0.125 m Tris HCl, pH 6.8), separated on 12% SDS/PAGE gel and immunoblotted with the indicated antibodies.
Expression and purification of recombinant HGAL protein
For expression and purification of Trx-HGAL fusion protein, BL21 (DE3) cells were transformed with pTRX-HGAL plasmid. Individual clones were grown at 37 °C in liquid broth containing 100 μg·mL−1 ampicillin until A600 of 0.6 was reached, followed by the addition of isopropyl thio-β-d-galactoside (final concentration 0.1 mm) for 3 h. The bacteria were collected and resuspended in a sonication buffer (10 mm Tris-HCl, 150 mm NaCl, pH 8.0) and lysed by sonication on ice. After 20 min of centrifugation at 12 000 g, the supernatant was applied to Ni2+ chelating Sepharose column (50/40 cm; Amersham Pharmacia Biotech; Sunnyvale, CA, USA) pre-equilibrated with starting buffer (50 mm Tris-HCl, 150 mm NaCl and 10 mm imidazole, pH 8.0), washed with washing buffer (50 mm Tris-HCl, 150 mm NaCl and 80 mm imidazole, pH 7.0) and then fusion protein was eluted using elution buffer (50 mm Tris-HCl, 150 mm NaCl and 200 mm imidazole, pH 7.0). The buffer of the eluate was changed to the strong anion ion exchange chromatography starting buffer (50 mm Tris-HCl, 20 mm NaCl, pH 8.0) and the solution was applied to a QFF Sepharose column (16/20; GE Healthcare Bio-Science Corp., Piscataway, NJ, USA). The proteins were eluted from the column with linear gradient of 1 m NaCl in starting buffer at 5 mL·min−1 constant speed for 100 min. Fractions containing the Trx-Src I fusion protein were pooled together.
Rabbit skeletal muscle myosin
Rabbit skeletal muscle myosin II was isolated and purified as described previously . Briefly, minced rabbit skeletal muscle was extracted in three volumes of ice cold Guba Straub buffer (0.1 m KH2PO4, 0.05 m K2HPO4 and 0.3 m KCl, pH 6.5) with constant stirring. The muscle mince was pelleted by centrifugation at 12 000 g for 30 min at 4 °C. The myosin containing supernatant was decanted and the myosin was precipitated using 13 volumes of ice-cold 1 mm EDTA. Precipitated myosin was collected by serial centrifugation at 8000 g for 10 min at 4 °C. The final spin was for 10 min at 12 000 g. The supernatant was removed and discarded. The myosin pellets were then dissolved in cold 20 mm Mops (pH 7), 1 mm dithiothreitol buffer and KCl to a final concentration of 0.5 m. Resuspended myosin was then ultracentrifuged at 125 000 g for 1.5 h at 4 °C. The myosin containing supernatant was then removed and precipitated a second time using 14 volumes of ice cold water. Myosin was collected by centrifugation at 4500 g for 10 min at 4 °C. After centrifugation, the supernatant was removed and discarded. Myosin pellets were left with a minimal volume of 1 mm dithiothreitol/water and stored overnight on ice. The next morning, myosin pellets were resuspended as described earlier in 20 mm Mops (pH 7), 1 mm dithiothreitol and 0.5 m KCl and ultracentrifuged again. The supernatant containing myosin was removed, mixed with glycerol in a 1 : 1 by volume ratio and stored at −20 °C until needed for the experiments.
Rabbit skeletal muscle actin was prepared as described previously  with modifications. Briefly, rabbit skeletal acetone powder was extracted with a G-actin buffer consisting of 2 mm Tris-HCl (pH 8.0), 0.2 mm Na2ATP, 0.5 mmβ-mercaptoethanol, 0.2 mm CaCl2 and 0.0005% NaN3 at a ratio of 20 mL·g−1 for 30 min with stirring on ice. The extract was centrifuged at 7000 g at 4 °C for 1 h to clarify and the tissue pellet was discarded. The supernatant was removed and adjusted to a final concentration of 40 mm KCl, 2 mm MgCl2 and 1 mm Na2ATP (pH 8.0). The F-actin was allowed to polymerize for 2 h at 4 °C. The KCl concentration was then increased again very slowly to a final concentration of 0.6 m and the solution was stirred slowly on ice for 30 min. This step was necessary to remove possible traces of tropomyosin–troponin. The F-actin was then collected by ultracentrifugation at 200 000 g at 4 °C for 1.5 h. The supernatant was discarded and the F-actin pellets were re-dissolved in a buffer consisting of 10 mm Mops (pH 7.0) and 40 mm KCl.
Labeling of F-actin with pyrene
For fluorescence assays, rabbit skeletal actin was labeled with pyrene lodoacetamide in accordance with the method described by Cooper et al. . Briefly, 20–40 μm F-actin was incubated at room temperature, in the dark, for 16 h with a 1.5 molar excess of N-(1-pyrene) iodoacetamide (Invitrogen) in a buffer containing 10 mm Mops (pH 7.0) and 40 mm KCl. Then the reaction was quenched with 1 mm dithiothreitol and the preparation was centrifuged at 200 000 g for 1.5 h. Next, F-actin was dialyzed against G-actin buffer (5 mm Tris-HCl, pH 8.0, 0.2 mm CaCl2, 0.2 mm ATP) to remove excess pyrene and dithiothreitol and polymerized overnight to form F-actin. The resulting molar ratio of pyrene/F-actin was 0.8 determined using the molar extinction coefficient, ε344(pyrene) = 22 000 m−1·cm−1.
Actin cosedimentation assay
Nonmuscle human actin (Cytoskeleton Inc., Denver, CO, USA) was diluted to 1 mg·mL−1 in a buffer containing 5 mm Tris (pH 8), 0.2 mm CaCl2, 0.2 mm ATP and 0.5 mm dithiothreitol, and centrifuged at 40 000 g for 10 min at 4 °C. The supernatant was used to induce actin polymerization by adding 50 mm KCl, 1 mm ATP and 2 mm MgCl2. The polymerization occurred at room temperature for 1 h. Recombinant HGAL protein was spun down at 100 000 g in a Beckman ultracentrifuge (Beckman Coulter, Fullerton, CA, USA) for 20 min at 22 °C. HGAL protein in the supernatant (0.01 and 0.02 mm) and F-actin (0.05 mm) were incubated in the buffer containing 10 mm Tris (pH 7.0), 1 mm ATP, 0.2 mm dithiothreitol, 1 mm EGTA, 0.1 mm CaCl2 and 2 mm MgCl2 for 1 h at room temperature, then spun at 100 000 g at 22 °C. The supernatants were carefully removed and 5× Laemmli SDS/PAGE sample buffer was added; 1× Laemmli SDS/PAGE sample buffer was added to the pellets. The pellets and supernatants were analyzed following their separation by SDS/PAGE and Coomassie Blue staining of the gel.
Myosin–HGAL cosedimentation assay
Rabbit skeletal muscle myosin was precipitated with 13 volumes of ice cold 1 mm dithiothreitol. Myosin was then collected by centrifugation at 8000 g for 10 min. The pellet was resuspended in a buffer containing 0.4 m KCl, 1 mm dithiothreitol and 10 mm Mops at pH 7 and dialyzed overnight. Myosin was diluted at a 1 : 11 ratio with 1 mm dithiothreitol and put on ice for 1 h. Recombinant HGAL protein was spun down at 100 000 g in a Beckman ultracentrifuge for 20 min at 22 °C. HGAL in the supernatant (0.01 and 0.02 mm) and myosin (0.05 mm) were mixed and incubated on ice for 30 min and then spun down at 100 000 g in Beckman ultracentrifuge for 30 min at 22 °C. The supernatants and pellets were carefully collected and analyzed following their separation by SDS/PAGE and Coomassie Blue staining.
Actin-activated myosin ATPase activity in the presence or absence of HGAL
The kinetics of the actomyosin interaction in the presence or absence of HGAL protein was measured using actin-activated myosin ATPase assays. Rabbit skeletal muscle myosin at the concentration of 1.9 μm was titrated with the increasing concentrations of rabbit skeletal F-actin (in μm): 0.1, 1, 2, 5, 10, 15, 20 and 25. The assays were performed in triplicate on 96-well microplates in a 120 μL reaction volume containing 25 mm imidazole (pH 7.0), 4 mm MgCl2, 1 mm EGTA and 1 mm dithiothreitol. The final salt (KCl) concentration was 0.107 m. The reactions were initiated with the addition of 2.5 mm ATP with mixing in a Jitterbug incubator shaker (Boekel, Feasterville, PA, USA) and allowed to proceed for 5 min at 30 °C and then terminated by the addition of 4% trichloroacetic acid. Samples were then centrifuged at 3720 g for 20 min and 50 μL of supernatants were transferred to the microplate for determination of inorganic phosphate by the Fiske–Subbarow method . Data were analyzed using the Michaelis–Menten equation, yielding the Vmax and KM parameters. In control experiments, pyrene-actin was titrated with myosin containing either HGAL-buffer with no HGAL added or BSA included in each titration point with myosin.
The effect of HGAL on the binding of myosin to F-actin
We used a fluorescence-based assay to examine the effect of HGAL on the binding of rabbit skeletal muscle myosin to pyrene-labeled F-actin. The measurements were performed in a 2 mL cuvette in a buffer containing 10 mm Mops, 0.4 m KCl (pH 7) using a Jasco FP-6500 Fluorometer (Jasco Inc., Easton, MD, USA). Pyrene-labeled F-actin at 0.5 μm, was titrated with the increasing concentrations of rabbit skeletal muscle myosin in the presence or absence of HGAL protein. Fluorescence was recorded at 408 nm with an excitation wavelength of 340 nm. The data were collected using felix software (Photon Technology International, Birmingham, NJ, USA) and fitted to a nonlinear binding model yielding apparent dissociation constants Kd .
The effect of HGAL on actin polymerization
Actin polymerization assay was performed using the Actin Polymerication Biochem Kit (Cytoskeleton Inc., Denver, CO, USA) in accordance with the manufacturer’s instructions. Briefly, pyrene-actin was added into the G-actin buffer (5 mm Tris-HCl, 0.2 mm CaCl2, 0.2 mm ATP, pH 8.0) and mixed with HGAL or just HGAL buffer (10 mm Mops, 40 mm KCl, 1 mm dithiothreitol, pH 7.0). The samples were read on a Spectra Max Gemini EM fluorescence microplate reader (Molecular Devices, Sunnyvale, CA, USA) at 60 s intervals for 120 cycles with excitation at 368 nm and emission at 430 nm.
In vitro motility assay
To examine the effect of HGAL on the interaction of actin and myosin at the molecular level, we utilized in vitro motility assays, as described previously . Briefly, a flow chamber was formed between a nitrocellulose coated coverslip and a standard glass slide with double-sided tape at the boundaries. Rabbit skeletal muscle myosin was introduced into the chamber in high salt buffer (300 mm KCl, 25 mm imidazole, 1 mm EGTA, 4 mm MgCl2, 1 mm dithiothreitol) and allowed to bind to the nitrocellulose surface for 2 min. Sixty microliters of 0.5 mg·mL−1 BSA in high salt buffer was then flowed through the chamber to remove any unbound myosin and block the remaining surface sites aiming to avoid nonspecific attachment of actin filaments or HGAL. After blocking, 60 μL of low salt buffer (25 mm KCl, 25 mm imidazole, 1 mm EGTA, 4 mm MgCl2, 1 mm dithiothreitol) was flowed through the chamber to remove any unbound BSA. Tetramethylrhodamine isothiocyanate labeled F-actin filaments (approximately 5 nm) in low salt buffer were added and allowed to bind to the myosin in the absence of ATP. Unbound actin was removed by washing with low salt buffer and movement was initiated by the addition of a low salt buffer with 1 mm ATP, scavenger (glucose oxidase, catalase and dextrose) and 0.5% methylcellulose. For some experiments, 30 μL of 400 μg·mL−1 HGAL was incubated for 5 min after the BSA blocking step and allowed to bind to the surface immobilized myosin.
Data were collected for several different loading concentrations of myosin. Filament movement was observed at 25 °C with an ICCD camera model IC200 (PTI, Birmingham, NJ, USA). Video sequences were captured using scion image and an AG-5 image grabber (Scion Corp, Frederick, MD, USA). The average velocity for a given filament was determined from the distance traveled by the filament between ten and 12 consecutive video images taken at intervals of 1 s using retrac (freeware software written by Dr Nick Carter, Warwick Medical School, The University of Warwick, Coventry CV4 7AL, UK). Fifteen to 25 filaments from each video segment were averaged and at least two video segments were obtained per flow cell.
Data are expressed as the mean ± SEM of n experiments. Comparisons between groups were performed using an unpaired Student’s t-test in sigma plot, version 11 (Systat Software, Inc., San Jose, CA, USA). P < 0.05 was considered statistically significant.
I.S.L. is supported by National Institutes of Health (NIH) grants NIH CA109335 and NIH CA122105, and the Dwoskin Family and Fidelity Foundations. D.S.-C. is supported by NIH grants HL071778 and HL090786. J.M. is supported by HL077280 and HL086655. D.M.H. is supported by the WCU Program through the National Research Foundation of Korea funded by the Ministry of Education Science and Technology (R31-2008-000-10071-0).
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