©1995 by The American Society for Biochemistry and Molecular Biology, Inc.
The Binding of Type I Collagen to Lymphocyte Function-associated Antigen (LFA) 1 Integrin Triggers the Respiratory Burst of Human Polymorphonuclear Neutrophils
ROLE OF CALCIUM SIGNALING AND TYROSINE PHOSPHORYLATION OF LFA 1 (*)

(Received for publication, April 11, 1995; and in revised form, July 31, 1995)

Roselyne Garnotel (1) Jean-Claude Monboisse (1)(§) Alain Randoux (1) Bernard Haye (2) Jacques Paul Borel (1)

From the  (1)Laboratory of Biochemistry, Faculty of Medicine, CNRS EP 0089, University of Reims, 51 rue Cognacq Jay, F 51095 Reims Cedex, France and the (2)Laboratory of Biochemistry, Faculty of Sciences, CNRS EP 0089, University of Reims, Moulin de la Housse BP 347, F 51062 Reims Cedex, France

ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
FOOTNOTES
ACKNOWLEDGEMENTS
REFERENCES

ABSTRACT

Monoclonal antibodies to the alpha(L)beta(2) integrin inhibit the binding of type I collagen to PMN (polymorphonuclear neutrophil leukocytes) as well as the subsequent stimulation of superoxide production and enzyme secretion elicited by this collagen. Pepsinized collagen still binds PMN but no longer stimulates them. The I domain of the alpha chain of the integrin is involved in the binding. Two sequences of the alpha(1)(I) polypeptide chain of collagen participate in the process. Experiments of competitive inhibition by synthetic peptides showed that the sequence RGD (915-917) is used for binding to the cells and DGGRYY (1034-1039) serves to stimulate PMN. Experiments of radioactive labeling of the cells and affinity chromatography on Sepharose-collagen confirmed the presence in PMN extracts of two proteins, 95 and 185 kDa, respectively, corresponding to the molecular weights of the beta(2) and alpha(L) chains of the integrin and recognized by their specific monoclonal antibodies.

The transduction pathways depending on the alpha(L)beta(2) integrin do not involve a G protein (ruled out by the use of cholera and pertussis toxins), whereas the cytoskeleton was found to participate in the process, as evidenced by inhibition by cytochalasin B. After collagen stimulation, cytoplasmic inositol trisphosphate and calcium ion increased sharply for less than 2 min. The use of the inhibitors staurosporine and calphostin C demonstrated that protein kinase C was involved. Evaluation of the activity of this enzyme showed that, upon stimulation of PMN with collagen I, it was translocated to plasma membrane.

Acrylamide gel electrophoresis of the protein bands corresponding to the integrin alpha(L)beta(2), followed by immunoblotting using monoclonal antibodies to phosphotyrosine, permitted us to demonstrate that, prior to stimulation by type I collagen, there was no phosphorylation, whereas after stimulation, both alpha(L)and beta(2) chains were stained by anti-phosphotyrosine antibodies. The adhesion of PMN to pepsinized type I collagen triggered tyrosine phosphorylation of the beta(2) chain of the integrin, without stimulating O&cjs1138;(2) production by these cells, whereas their stimulation by complete type I collagen induced the tyrosine phosphorylation of both alpha(L) and beta(2) subunits. The tyrosine phosphorylation of both integrin subunits during transduction of stimuli is a heretofore undescribed phenomenon that may correspond to a new system of transmembrane communication.


INTRODUCTION

Type I collagen, a major component of the extra cellular matrix, promotes the adhesion of a variety of cells in solid tissues, influencing many processes such as proliferation, differentiation, migration, and cell shape changes(1) . Several receptor molecules have been demonstrated as promoting the adhesion to type I collagen. Among these receptors, some belong to the family of integrins, for instance alpha(1)beta(1), alpha(2)beta(1), and alpha(3)beta(1)(2) . On the other hand, some types of mobile cells also interact with collagens, for instance polymorphonuclear neutrophils (PMN),^1 a variety of leukocytes circulating in blood, capable of crossing the vascular wall in order to invade the inflamed tissues and to participate in defenses against bacteria or foreign molecules through their property of phagocytosis. In several previous papers, we demonstrated that PMN and type I collagen do interact and began to describe their interactions (3, 4, 5) .

Purified type I collagen is able to bind to PMN in vitro. This binding is followed by the stimulation of some main functions of PMN, such as emission of pseudopods, secretion of lytic enzymes, and liberation of superoxide. We demonstrated that the stimulation of PMN by collagen occurs through two sequences of the alpha(1)(I) chain, both located in the C-terminal region of the molecules, an RGD sequence corresponding to residues 915-917, and a DGGRYY sequence corresponding to residues 1034-1039, located at the C-terminal extremity of the chain. The type I collagen molecule, either fibrillar or denatured, is active, whereas pepsinized collagen, lacking the C-terminal telopeptide, is not. The cyanogen-bromide cleaved peptide alpha1(I)-CB6, which contains the C-terminal residues (823-1039) of the alpha(1) chain, is also active. In contrast, the addition of the peptides RGD and DGGRYY either separately or together induces an inhibition of PMN. Both sequences must be contained in the same peptidic molecule to remain active on PMN.

By using monoclonal antibodies, we were able to demonstrate that the beta(2) chain of the integrins is involved in the process of binding of PMN onto type I collagen. The main integrins already found in the membrane of PMN all belong to the group of beta(2) integrins and are alpha(L)beta(2) (also termed CD11a-CD18, LFA 1), alpha(M)beta(2) (CD11b-CD18 or Mac 1), and alpha(X)beta(2) (CD11c-CD18, p150-95).

The aim of this paper is to demonstrate that the receptor of type I collagen is the integrin alpha(L)beta(2), that this integrin mediates not only the binding but also transduction of the stimulation message, and that this phenomenon depends on the tyrosine-phosphorylation of both the alpha(L) and beta(2) subunits. We also point out some new details on the system of transduction operating intracellularly beyond the receptor.


EXPERIMENTAL PROCEDURES

Materials

Type I collagen was prepared from rat tail tendon by 0.1 M acetic acid extraction(6) . Ferricytochrome c (type VI), superoxide dismutase from bovine erythrocytes, bovine serum albumin, fMet-Leu-Phe, pertussis toxin, cholera toxin, cytochalasin B, lactoperoxidase, H-7 (1-(isoquinolenylsulfonyl)-2-methylpiperazine), staurosporine, were all purchased from Sigma. Calphostin C was bought from Calbiochem (La Jolla, CA). The following monoclonal antibodies were used: P4C10, recognizing the beta1 integrin subunit (Life Technologies, Inc.); 4-G7, raised toward the lymphocyte surface antigen Leu-12, D-12, recognizing CD11b, and 5-HCl-3, recognizing CD11c, all from Becton-Dickinson (Mountain View, CA); MHM-24, raised against CD11a, MHK-23, recognizing CD18 from Dakopatts (Glosdrup, Denmark); MEM-25, Bear-1, FK-24, and MEM-48, recognizing CD11a, CD11b, CD11c, CD18, respectively, from Monosan (Tebu, Paris, France). Monoclonal antibodies to phosphotyrosine (clone 6G9, Life Technologies; and PY 20, Calbiochem) were used.

The synthetic peptides GRGD, DGGRYY, RFDS, CGRGDSPC, and CGRGESPC were synthesized by Neosystem (Strasbourg, France). Fura-2 was bought from Molecular Probes Inc (Eugene, OR). NaI and [^3H]inositol were from DuPont NEN.

Preparation of PMN

Human blood was obtained on consent from healthy subjects. PMN were isolated according to a previously published method (4) involving a single-step centrifugation procedure through a Metrizoate-Polyprep gradient (Nycomed, Oslo, Norway) at 240 times g for 35 min at room temperature. The PMN-rich layer was drawn, washed once in Dulbecco's solution, pH 7.4, and centrifuged at 600 times g for 15 min at room temperature. The contaminating erythrocytes were eliminated by hypotonic lysis in 15 mM ammonium chloride. The cells were finally suspended at 10^7/ml in Dulbecco's solution, pH 7.4, containing 1.3 mM Ca and 0.5 mM Mg, at 4 °C. The percentage of PMN in cell preparations exceeded 95%, and the cell viability, as determined by trypan blue exclusion, was over 98%.

Experiments of Cell Adhesion

Polystyrene 96-well plates (Nunc, Copenhagen, Denmark) were coated with type I collagen solubilized in 0.1 ml of 0.018 M acetic acid solution at a concentration of 50 µg/well. The protein-containing plates were washed three times with 150 mM NaCl prior to the addition of 1.5 times 10^5 cells in 100 µl of Dulbecco's solution containing 1.3 mM Ca and 0.5 mM Mg. After a 30-min incubation period, the non-adherent cells were discarded. The adherent cells were fixed with 100 µl of a 1.1% (v/v) glutaraldehyde solution for 15 min. After extensive washing with distilled water, 0.1 ml of crystal violet solution (100 mg/100 ml in 0.2 M Hepes buffer, pH 6.0) was added to every well, left for 15 min, and discarded. The adhesion of PMN was evaluated spectrophotometrically as the absorbance of the stained nuclei at 560 nm, according to Kueng(7) .

Measurement of Superoxide Ion (O&cjs1138;(2))

The O&cjs1138;(2) release was measured from the superoxide dismutase-inhibitable reduction of ferricytochrome c, according to English(8) . The PMN suspension (10^6 cells in 100 µl) was added to a small glass test tube containing 0.1 ml of 1 µM cytochrome c solution and 0.85 ml of Dulbecco's solution. O&cjs1138;(2) release was induced by adding 0.1 ml of the activating agent solution (either fMet-Leu-Phe at the concentration 0.1 µM in saline or 0.3 µM type I collagen in 0.018 M acetic acid solution). The increase in absorbance was followed spectrophotometrically as an index of the amount of liberated superoxide. Test tubes supplemented with 0.05 ml of superoxide dismutase solution in saline were taken as blanks assessing the specificity of the reaction.

Measurement of Granule Secretion

A 0.1-ml aliquot containing 10^6 PMN was added to 0.8 ml of Dulbecco's solution and 0.1 ml of collagen solution (final concentration 0.3 µM) already mixed in a glass test tube. The mixture was incubated for 30 min at 37 °C. Cells were then removed by centrifugation at 800 times g for 5 min and the enzymatic activities measured in the supernatant.

The evaluations of elastase and of 92-kDa type IV collagenase were performed using N-methoxysuccinyl-Ala-Ala-Pro-Val-p-nitroanilide and biotinylated type IV collagen as substrates, for incubation periods of 1 and 3 h, respectively, according to the methods of Nakajima et al.(9) and of Wilkinson et al.(10) . The N-acetyl-beta-D-glucosaminidase activity was measured according to the method of Troost et al.(11) . Lactic dehydrogenase, whose evaluation permits to verify the absence of cell lysis, was evaluated as described by Buhl et al.(12) . The enzymatic activities released in the medium were expressed as percentage of the corresponding total activity of the cell lysate.

Effect of Monoclonal Antibodies on PMN

Treff polypropylene microtubes (Polylabo, Strasbourg, France) were coated with 1.5 ml of fetal calf serum (Life Technologies) by agitation at 37 °C for 1 h and then extensively washed with a 0.15 M NaCl solution. A 0.1-ml volume of antibody solution, at the appropriate titer, was added to each tube, followed by the PMN suspension in Dulbecco's solution, in order to achieve a final concentration of 6 times 10^6 cells in 0.75 ml. Test tubes were shaken horizontally in a mechanical shaker for 90 min at 150 cycles/min (13) .

Affinity Chromatography

Ten mg of purified type I collagen were covalently coupled to 1 ml of packed beads of CNBr-activated Sepharose 4B (Pharmacia Biotech Inc.) according to the manufacturer's instructions. In parallel, a suspension of 20 times 10^6 cells in 1.5 ml of phosphate-buffered saline was iodinated using the lactoperoxidase method of Lebien et al.(14) . Iodination was carried out on ice by addition of 200 µg of lactoperoxidase followed by 37 MBq of NaI dissolved in 0.1 ml of water and two additions of 20 µl of 0.12% (w/v) hydrogen peroxide at a 5-min interval. Reaction was terminated by adding 2 ml of ice-cold phosphate-buffered saline, and the cells were washed three times with this solution. The cells were then extracted in 1 ml of a 100 mM Tris-HCl buffer pH 7.4, containing 150 mM NaCl, 0.5% (w/v) Nonidet P-40, 0.1% (w/v) sodium dodecyl sulfate (SDS), 1% aprotinin (w/v), 2 mM phenylmethylsulfonyl fluoride, 10 µg/ml leupeptin. Following clarification by centrifugation at 12,000 times g for 15 min at 4 °C, the lysate was diluted 1/5 with a 10 mM Tris-HCl buffer pH 7.4 containing 1.3 mM CaCl(2), 1 mM MgCl(2), 1 mM benzamidine, 2 mM phenylmethylsulfonyl fluoride, 10 µg/ml leupeptin. This dilution was necessary to reduce the concentration of Nonidet P-40 and SDS. The extract was transferred onto the collagen-Sepharose 4B beads in batch and incubated overnight in the same conditions. The suspension was then packed into a 1.0-cm diameter glass column and washed at 4 °C by buffer A at a flow of 5 ml/h.

The bound material was eluted first with a 10 mM Tris-HCl buffer, pH 7.4, containing 5 mM EDTA, 0.1% (w/v) n-octyl beta-D-glucopyranoside, 150 mM NaCl, 1 mM benzamidine, 2 mM phenylmethylsulfonyl fluoride, 10 µg/ml leupeptin, at a rate of 1 ml/h, then with the same buffer containing 1.0 M NaCl in the place of 150 mM. In some instances, the proteins were sequentially eluted by the specific peptides, first by 4 ml of a 3 mM solution of synthetic DGGRYY, then by 4 ml of a 3 mM solution of CGRGDSPC. Both peptides were dissolved in a 10 mM Tris-HCl buffer, pH 7.4, containing 0.1% (w/v) n-octyl beta-D-glucopyranoside, 150 mM NaCl, 1 mM benzamidine, 2 mM phenylmethylsulfonyl fluoride, 10 µg/ml leupeptin.

Fractions of 1 ml were collected and their radioactivity counted with an automatic counter (Kontron MR-480) in order to monitor the elution. For characterization of the eluted substances, the proteins contained in 200-µl aliquots corresponding to the peaks of radioactivity were precipitated by addition of ethanol to 80% (v/v). The precipitates were redissolved in Laemmli sample buffer (15) and submitted to electrophoresis in a 7.5% polyacrylamide gel under reducing conditions. Radioactive bands were revealed by exposure to a Hyperfilm MP (Amersham Corp.) for convenient periods of time.

Immunoprecipitations

Aliquots of 200 µl of the eluted fractions were coupled to the monoclonal antibodies and to protein A-Sepharose by incubation at 4 °C for 2 h. The Sepharose-adsorbed material was washed three times with 3 ml of Tris-buffered saline. The eluted proteins were analyzed by SDS-PAGE under reducing conditions and detected by autoradiography as described above(16) .

Preincubation of PMN with Specific or Competitive Inhibitors

PMN were incubated for 10 min at 37 °C either with pertussis toxin (final concentration 100-500 ng/ml), with cholera toxin (2.5 µg/ml), with cytochalasin B (2.5 µg/ml), with the protein kinase C inhibitors staurosporine (0-500 nM), H-7 (0-1000 µM), calphostin C (0-500 nM), or with the inhibitor of tyrosine kinase genistein (0-2.0 µg/ml). After this preincubation, they were stimulated by addition of 0.1 µM fMet-Leu-Phe or of 0.3 µM collagen I. The production of superoxide was evaluated by spectrophotometry of the superoxide dismutase-inhibitable reduction of cytochrome c as indicated above.

In another series of experiments, PMN were preincubated for 15 min at 37 °C with the synthetic peptides RFDS, GRGD, CGRGDSPC, CGRGESPC, or DGGRYY at various concentrations. At the end of this incubation, they were stimulated by addition of 0.3 µM collagen I. The O&cjs1138;(2) production and enzyme-rich granule release were evaluated as described above.

Intracellular Calcium Ion Measurement

The intracellular Ca concentration was measured according to Grynkiewicz et al.(17) . A suspension of PMN (10^7/ml), in a Dulbecco's solution containing 1.3 mM CaCl(2), 0.5 mM MgCl(2) and 10 mM glucose, was loaded with 0.5 µM Fura-2-AM for 30 min at 37 °C, rinsed twice with Dulbecco's solution, and sedimented. The cells were resuspended in Dulbecco's solution at an amount of 10^7 cells/ml. Two ml of this suspension were transferred into the cuvette of a Shimadzu RF 5000 spectrofluorometer. The apparatus was set up at two excitation wave lengths of 340 and 380 nm, and the emitted fluorescence monitored at 510 nm for 3 min in order to determine the basal level, the stimulating agent (final concentration 0.1 µM fMet-Leu-Phe or 0.3 µM type I collagen) was added and fluorescence recorded for 10 min. At the end of each experiment, cells were lysed by adding a 0.1% (w/v) Triton X-100 solution and the maximal fluorescence measured. Minimal fluorescence was also determined after addition of 2.0 mM MnCl(2) solution. Results were expressed as nanomoles of Ca/10^7 cells.

Intracellular Inositol Trisphosphate Measurement

PMN were suspended at a concentration of 10^7 cells/ml in Dulbecco's solution containing 0.0025% (w/v) bovine serum albumin and were incubated with 1.11 MBq of [^3H]inositol for 120 min at 37 °C. Ten minutes before the end of this incubation, 1 ml of a solution of 10 mM LiCl(2) was added in order to inhibit the hydrolysis of inositol phosphate. Finally, the cells loaded with [^3H]inositol were rinsed twice with Dulbecco's solution containing 10 mM LiCl(2) and resuspended at 2 times 10^7 cells/ml in fresh Dulbecco's solution.

The experiment was performed after several types of stimuli had been applied to the cells, either 0.1 µM fMet-Leu-Phe or 0.3 µM type I collagen. The incubation was stopped at various times (0, 0.5, 1.0, 2.0, or 5.0 min) by addition of 0.15 ml of a 35% (w/v) sodium perchlorate solution. The reaction mixture was centrifuged at 5,000 times g for 15 min at 4 °C. The supernatants were neutralized with a 9.0 M KOH solution and deposited at the top of columns of Dowex AG-1X8 (200-400-mesh) equilibrated under the formate form. The column was eluted sequentially with 3 ml of distilled water (for free [^3H]inositol), 10 ml of 5 mM sodium tetraborate/60 mM sodium formate (for glycerophospho[^3H]inositol), 14 ml of 0.1 M formic acid/0.2 M ammonium formate (for [^3H]inositol phosphate), 18 ml of 0.1 M formic acid/0.5 M ammonium formate (for [^3H]inositol bisphosphate), 18 ml of 0.1 M formic acid/1.0 M ammonium formate (for [^3H]inositol trisphosphate), according to the method of Berridge(18) . The radioactivity of the eluted fractions was measured in a Packard 1900 TR liquid scintillation counter. Results were expressed as percentage of total inositol phosphate.

Measurement of Protein Kinase C Activity

Protein kinase C activity was evaluated in the particular or in the cytosolic fractions of PMN stimulated with fMet-Leu-Phe, PMA, or type I collagen, according to the method described by Kikkawa et al.(19) .

Tyrosine Phosphorylation of the alpha(L)beta(2)Integrin

The suspension of PMN (10^7 cells/ml) in Dulbecco's solution containing 1.3 mM CaCl(2), 0.5 mM MgCl(2), was first preincubated for 30 min at 20 °C in the presence of 2.5 mM phenylmethylsulfonyl fluoride. Then temperature was raised to 37 °C for 5 min prior to the addition of the stimulating agent (Dulbecco's solution as a control, 0.1 µM fMet-Leu-Phe peptide in Dulbecco's solution, or 0.3 µM type I collagen in Dulbecco's solution). The incubation was stopped after 2 min by centrifugation at 1000 times g for 4 s at 4 °C. The supernatants were discarded and the cells lysed by addition of 150 µl of a 0.05 M Hepes buffer, pH 7.5, containing 150 mM NaCl, 5 mM EGTA, 10 mM sodium pyrophosphate, 10 mM sodium fluoride, 5 mM orthovanadate, 1% (w/v) SDS, 1% (w/v) Nonidet P-40, 10% (w/v) glycerol, and a mixture of proteinase inhibitors (1 mM phenylmethylsulfonyl fluoride, 10 µg/ml aprotinin, 10 µg/ml leupeptin, and 1 µM pepstatin A)(20) . Cell lysis took place within 10 min at 4 °C.

A 100-µl aliquot of cell extract was immunoprecipitated by addition of anti-CD18 or anti-CD11a monoclonal antibodies (6 µg/ml), followed by adsorption on protein A-Sepharose for 2 h at 4 °C. The immunoprecipitated material was fractionated by SDS-PAGE in 10% polyacrylamide gel under reducing conditions and blotted on a transfer Immobilon membrane (Millipore, Bedford, MA). The membrane was saturated by incubation for 1 h with a 10 mM Tris buffer, pH 7.4, containing 150 mM NaCl and 5% (w/v) bovine serum albumin, then incubated for 2 h in the presence of monoclonal antibodies to phosphotyrosine (clone 6G9 or clone PY-20). Alkaline phosphatase-conjugated anti-mouse IgG antibody (Organon Teknika, Durham, NC) was used as a second antibody, for detection of the positive protein bands visualized by the reaction with 5-bromo-4-chloro-3-indolyl phosphate in the presence of nitro blue tetrazolium.

For the evaluation of tyrosine phosphorylation of the alphaLbeta2 integrin subunits, PMN (5 times 10^7 cells) were labeled with 18.5 MBq of PO(4)H(3) for 30 min and then incubated with 0.3 µM type I collagen (pepsinized or not). The membrane extracts were immunoprecipitated with anti-CD18 or anti-CD11a antibodies, and the immunoprecipitated material was analyzed by SDS-PAGE. The integrin subunits were submitted to an alkaline treatment prior to 5.7 M HCl hydrolysis. Phosphoamino acids were derivatized with 9-fluorenylmethylchloroformate (Fmoc) according to (21) , and the Fmoc-derivatives were analyzed by reverse phase high performance liquid chromatography on an Hypersil RP 18 (5 µm) column.


RESULTS

Identification of the Sequences of Type I Collagen Responsible for Adhesion and Stimulation

Preparations of PMN were submitted to the effect of solutions of synthetic peptides containing sequences RGD and DGGRYY. After a 15-min treatment, an aliquot of cells was added onto type I collagen molecules layered to the bottom of the wells of culture polystyrene plates. Adhesion to collagen and production of O&cjs1138;(2) by these cells were measured (Table 1). The linear peptide GRGD and the control peptide RFDS did not exert any significant action. On the other hand, the peptide CGRGDSPC, which contains RGD in a loop formed under the influence of a disulfide bridge, exerted an inhibiting effect of about 50% on both adhesion and superoxide production, whereas peptide CGRGESPC did not. This effect was slightly dose-dependent. Peptide DGGRYY did not inhibit the binding of PMN to type I collagen but inhibited the formation of O&cjs1138;(2) in a dose-dependent manner. The secretion by PMN of lytic enzymes such as elastase or gelatinase was found to be inhibited by the peptides CGRGDSPC or DGGRYY in parallel to superoxide liberation (Table 2).





Identification of LFA 1 as the Receptor for Type I Collagen on PMN Membrane

In experiments similar to the previous one, monoclonal antibodies to the various subunits of the beta(2) integrins were incubated with PMN, then the adhesion of the cells was measured as well as superoxide secretion (Table 3) and granule exocytosis (Table 4). Two monoclonal antibodies recognizing the beta(2) chain of integrins, MHM 23 and MEM 48, were found to inhibit both adhesion of PMN to collagen and secretions of superoxide and lytic enzymes. On the other hand, one of the monoclonal antibodies recognizing the alpha(L) chain, MEM 25, inhibited both adhesion and stimulation of the cells, whereas the second monoclonal antibody to the alpha(L) chain did not induce any inhibition. The secretions of lytic enzymes by PMN, such as elastase or gelatinase induced by type I collagen, were found to be inhibited by the same monoclonal antibodies as superoxide liberation. The monoclonal antibodies inhibited the secretions by PMN in a dose-dependent manner (Fig. 1). None of the monoclonal antibodies recognizing alpha(M) or alpha(X) chains inhibited adhesion or activation of PMN.






Figure 1: Dose-dependent inhibiting effect of monoclonal antibodies to the integrin subunits alpha(L) and beta(2) on the PMN adhesion to collagen (A) and on the superoxide production triggered by type I collagen (B). A first incubation of 6 times 10^6 PMN was performed for 90 min in the presence of monoclonal antibodies anti-CD11a (clone MEM 25, bullet) or anti-CD18 (clone MEM 48, &cjs2108;), and then an aliquot of these cells (1.5 times 10^5) was layered on a type I collagen-coated plate and their adhesion measured by nuclei staining with crystal violet. Another aliquot (1 times 10^6) was incubated for 15 min with type I collagen in a test tube in order to measure the production of superoxide by the superoxide dismutase-inhibitable reduction of ferricytochrome. Bars represent 1 S.D. from the mean.



Isolation of the Receptor

The isolation of the receptor membrane protein was undertaken by the method of affinity chromatography on a column of type I collagen-Sepharose. The elution diagram is shown on Fig. 2. Two peaks were found, one eluted with buffer A containing 5 mM EDTA and 150 mM NaCl and the second with the same buffer A containing 1 M NaCl.


Figure 2: Elution profile of the affinity chromatography of a PMN extract performed on type I collagen-Sepharose. The left arrow represents the start of elution by 150 mM NaCl + 5 mM EDTA. The right arrow represents the start of elution by 1 M NaCl + 5 mM EDTA. Inset, characterization by SDS-PAGE of the fractions eluted from the affinity column of collagen-Sepharose. Electrophoresis carried out in 7.5% polyacrylamide gel at pH 8.3. Detection by autoradiography. Lane 1, molecular size standards revealed by Coomassie Blue; lane 2, total extract from iodinated membrane; lane 3, peak 1; lane 4, peak 2.



SDS-PAGE was performed on the proteins contained in both peaks (Fig. 2, inset). The first peak of elution contained two major bands with respective apparent molecular masses of 95 and 185 kDa as estimated by comparison to control globular proteins of known molecular mass. In addition, this peak contained two minor bands, of 31 and 35 kDa, respectively. Peak two contained these 31- and 35-kDa proteins as major bands.

The identity of the proteins contained in these peaks was verified by immunoprecipitation with the monoclonal antibodies anti-CD18 and anti-CD11a. The precipitated molecules were analyzed by SDS-PAGE. The antibody anti-CD18 precipitated the two proteins of molecular masses 95 and 185 kDa from peak 1 (Fig. 3A). No material from peak 2 was precipitated by this antibody. Similar results were obtained with the antibody anti-CD11a (Fig. 3B). Monoclonal antibodies to CD11b and CD11c did not precipitate any material.


Figure 3: SDS-PAGE of the immunoprecipitates. A, obtained with the monoclonal antibody to CD18. Lane 1, peak 1 from the affinity chromatography; lane 2, peak 2. B, obtained with the monoclonal antibody to CD11a. Lane 1, peak 1 from the affinity chromatography; lane 2, peak 2.



The synthetic peptides CGRGDSPC and DGGRYY used either separately or together were not able to elute significant amounts of proteins from the column by themselves (data not shown).

Further Steps of Transduction of the Message beyond the Receptor: G Proteins

The necessity of a G(s) protein for transduction of the message was checked by addition of cholera toxin to the preparation of PMN and measurement of the production of superoxide in the presence of type I collagen. No influence of this toxin was noticed either on collagen-stimulated PMN or on control fMet-Leu-Phe-stimulated PMN (data not shown).

In the same type of experiments, the effect of pertussis toxin (at concentrations ranging from 0 to 500 ng/ml) on the collagen-dependent formation of superoxide was compared to the effect of this toxin on the fMet-Leu-Phe-dependent stimulation. Pertussis toxin was found to be inactive on the transduction of the message from type I collagen, whereas it exerted a dose-dependent inhibiting effect on the stimulation by the peptide fMet-Leu-Phe used as a control.

Effect of Cytochalasin B and Colchicine on the Production of Superoxide

These inhibitors of cytoskeleton assembly were added to PMN at concentrations 2.5 µg/ml and 10M, respectively, 10 min prior to stimulation by addition of type I collagen or control fMet-Leu-Phe. The result of this addition on the production of superoxide by the cells was measured (Table 5). While cytochalasin B or colchicine increased the production of superoxide in the presence of fMet-Leu-Phe, they suppress this effect in the presence of type I collagen. Similar results were obtained when measuring granule exocytosis (data not shown).



Inositol Trisphosphate

The results of the evaluation of the inositol trisphosphate in the cytoplasm of PMN after various stimulations are shown on Fig. 4. There was a fast rise in the concentration of inositol trisphosphate, with a peak about 0.5 min after the onset of stimulation in the case of the use of type I collagen or peptide fMet-Leu-Phe, whereas in the case of treatment with pepsinized type I collagen the amount of inositol trisphosphate remained comparable to the base-line levels obtained with Dulbecco's solution as a control. Preincubation of PMN with monoclonal antibodies anti-CD11a or anti-CD18 inhibited the rise in the concentration of inositol trisphosphate triggered by collagen I, without affecting that induced by fMet-Leu-Phe.


Figure 4: Variations of the cytoplasm content of inositol trisphosphate under various stimuli. PMN (5 times 10^7 cells/ml) were preincubated for 120 min at 37 °C in the presence of [^3H]inositol (1.11 MBq/ml), and then aliquots of 10^7 cells were stimulated either with control Dulbecco's solution, with 0.1 µM fMet-Leu-Phe, 0.3 µM type I collagen, or 0.3 µM pepsinized type I collagen. Inositol trisphosphate was evaluated as described under ``Experimental Procedures.'' Data represent the mean of quadruplicate determinations.



Calcium Ion

The results of the evaluation of calcium ion concentrations in the cytoplasm of PMN are shown on Fig. 5. Once again, type I collagen elicited a sudden rise of the calcium concentration, comparable to that elicited by the control peptide fMet-Leu-Phe, followed by a decrease within 2 min after the onset of stimulation. Pepsinized collagen was inactive. On the other hand, preincubation of PMN with monoclonal antibodies anti-CD11a or anti-CD18 inhibited the calcium mobilization triggered by collagen I without affecting that induced by fMet-Leu-Phe (data not shown).


Figure 5: Increase of the cytoplasmic free Ca concentration. PMN were loaded for 30 min with Fura-2. The vertical arrow shows the instant of addition of stimulating agent. A, Dulbecco's solution as a control. B, 0.1 µM fMet-Leu-Phe solution. C, 0.3 µM pepsinized type I collagen. D, 0.3 µM type I collagen.



Protein Kinase C

The participation of protein kinase C in the process was tested with three inhibitors: H-7, staurosporine, and calphostin C. The first inhibitor had no effect on the production of superoxide by PMN stimulated by collagen (whereas under the same conditions it decreased this formation when induced by contact with peptide fMet-Leu-Phe) (Fig. 6). Staurosporine and calphostin C decreased the stimulation exerted by type I collagen in a concentration-dependent manner parallel to that induced by the control peptide fMet-Leu-Phe but in greater proportion (Fig. 6). The stimulation of PMN with collagen I triggered the translocation of protein kinase C from cytosolic to particular fraction as fMet-Leu-Phe or PMA did (Fig. 7).


Figure 6: Effect of the protein kinase C inhibitors on superoxide production by PMN. A, inhibition by H-7; B, inhibition by staurosporine; C, inhibition by calphostin C. An amount of 10^6 cells was preincubated for 10 min at 37 °C in the presence of the protein kinase C inhibitor and then stimulated with 0.3 µM collagen (bullet) or 0.1 µM fMet-Leu-Phe (). Data represent mean of quadruplicate determination. Bars represent 1 S.D. from the mean.




Figure 7: Protein kinase C activity of the PMN. The activity of protein kinase C was measured in the cytosolic (light shaded bars) and in the particular (darker shaded bars) fractions of PMNs stimulated with: 1, Dulbecco's solution alone (control); 2, 0.3 µM collagen I; 3, 0.1 µM fMet-Leu-Phe; 4, 8 nM PMA. Protein kinase C was measured 2 min after stimulation. Data represent mean of triplicate determinations. Bars represent 1 S.D. from the mean.



Effect of Genistein

The stimulation of the production of superoxide by type I collagen and by the peptide fMet-Leu-Phe was found to be decreased by this inhibitor of protein tyrosine kinase (Fig. 8).


Figure 8: Inhibitory effect of genistein on superoxide production triggered by PMN. PMN (10^6 cells) were preincubated for 10 min with genistein and then stimulated with 0.3 µM type I collagen (bullet) or with 0.1 µM peptide fMet-Leu-Phe (). The release of superoxide was measured through the superoxide dismutase-inhibitable reduction of ferricytochrome c. Data represent mean of quadruplicate determinations. Bars represent 1 S.D. from the mean.



Detection of the Tyrosine Phosphorylation of the Subunits of Integrin alpha(L)beta(2)

After stimulation of PMN by type I collagen, the proteins extracted from plasma membrane have been precipitated by anti-CD18 or anti-CD11a monoclonal antibodies. Fig. 9shows that the precipitated proteins, analyzed by SDS-PAGE, migrate with electrophoretic mobilities identical to that of the alpha(L) and beta(2) subunits. Immunoblotting by an antibody to phosphotyrosine was inhibited by an excess of free phosphotyrosine. The electrophoregram showed that a tyrosine-phosphorylation of the beta(2) subunit of the integrin was taking place in case of adhesion of PMN to pepsinized type I collagen, whereas stimulation by complete collagen induced the tyrosine-phosphorylation of both alpha(L) and beta(2) subunits. Phosphoamino acid analysis confirmed the presence of P-labeled phosphotyrosine in the beta(2)-integrin subunit in PMN incubated with pepsinized type I collagen, and in both alpha(L) and beta(2) subunits in PMN stimulated with complete type I collagen.


Figure 9: Tyrosine phosphorylation of the alpha(L)beta(2) integrin subunits after PMN stimulation. SDS-PAGE of the membrane proteins precipitated by anti-CD18 (lanes 1-5) or with anti-CD11a (lanes 6 and 7) and stained by an antibody to phosphotyrosine. Incubation of PMN for 2 min with Dulbecco's solution alone (lane 1), bovine serum albumin (lane 2), 0.1 µM fMet-Leu-Phe (lanes 3 and 7), 0.3 µM acid-soluble collagen I (lanes 4 and 6), and 0.3 µM pepsinized collagen I (lane 5).




DISCUSSION

The alpha1(I) chain of type I collagen stimulates PMN functions such as respiratory burst and degranulation through two distinct sequences, an RGD sequence corresponding to residues 915-917 and a DGGRYY sequence corresponding to the C-terminal extremity of this polypeptide chain, residues 1034-1039(4) .

The synthetic CGRGDSPC peptide, which exposes the RGD sequence on a loop, inhibits the adhesion of PMN to type I collagen, whereas linear GRGD and CGRGESPC do not. The conformation of RGD sequences is critical for fulfilling its function of fixation or message transmission(22) . The peptide DGGRYY does not inhibit the binding of type I collagen to PMN, whereas it inhibits superoxide and lytic enzyme secretions. The functions of binding and stimulating are distributed between the two peptide sequences involved in the ligand. Apparently, RGD, when correctly folded, is in charge of binding, whereas DGGRYY is responsible for the transmission of stimulation. Pepsinized alpha(1)(I) chain of collagen I, which does not contain the sequence DGGRYY, still binds PMN, but this binding is not followed by stimulation. It must be noted that the binding of PMN onto type I collagen seems necessary for the stimulation to occur but that a specific inhibition of the stimulation may occur independently of the binding. Finally, this binding also necessitates the presence of Mg and Ca ions, as we have already demonstrated(5) .

Previously we found that a beta(2) integrin is involved in the stimulation of PMN by type I collagen(5) , but we had not yet identified the alpha chain. In this paper, we demonstrate that the membrane receptor of type I collagen on PMN is constituted by integrin alpha(L)beta(2) (LFA 1). The adhesion of PMN to type I collagen is abolished by a preliminary treatment of the cells with two monoclonal antibodies to the beta(2) chain (clones MHK 23 and MEM 48) by about 95%.

Two monoclonal antibodies (clones MEM 25 and MHM 24) had been used to immunoprecipitate the alpha(L) chain and the recombinant I domain(23) . Surprisingly, in our experiments, the MHM 24 antibody did not inhibit the adhesion of PMN to collagen I, whereas MEM 25 did. This discrepancy may depend on the fact that the epitope recognized by the MHM 24 antibody is too distant from the domain of collagen binding, as documented in (24) .

The properties of the inhibiting antibody MEM 25 suggest that the I domain of alpha(L) chain is involved in the adhesion of PMN to collagen. The I domain is present in the alpha chains of the beta(2) group of integrins as well as in the alpha(2) chain of the alpha(2)beta(1) integrin, which is a receptor for collagen in various cells(25) . This domain may represent a common marker for the adhesion of type I collagen, despite the restricted level of identity (36%) between the three alpha chains of beta(2) integrins(26) . Other authors suggested the adhesion of PMN to collagen I through the alpha(M)beta(2) integrin(27) .

Characterization of the receptor protein by radioactive iodine labeling of whole cells, followed by preparation of plasma membranes and affinity chromatography of proteins on Sepharose-type I collagen columns, permitted isolation of two major peaks. In SDS-PAGE, peak 1 was found to contain two protein bands of 95 and 185 kDa, respectively, apparent molecular masses corresponding to those proposed in literature for beta(2) and alpha(L) chains (16) . The identity of the two chains was assessed by immunoprecipitation of the fractions with anti-beta(2) and anti-alpha(L) monoclonal antibodies. Anti-alpha(M) and anti-alpha(X) monoclonal antibodies were devoid of effect. In addition, peak 1 contained traces of two other proteins, whose apparent molecular masses, as estimated by SDS-PAGE, corresponded to 31 and 35 kDa. We have no information on their nature and relationship with the alpha(L)beta(2) integrin.

As regards the transduction pathways linking the membrane receptor of type I collagen to the effector systems of superoxide formation and enzyme granule secretion, neither G(s) nor G(i) proteins were involved (absence of effect of cholera and pertussis toxins). The final result of PMN stimulations by the bacterial peptide fMet-Leu-Phe and by type I collagen is the same, but the former depends on a G(i) protein associated to a seven-transmembrane domain receptor, whereas the second depends on the alphaLbeta2 integrin; one can question at which point the transduction pathways for both systems become identical.

Cytochalasin B, an inhibitor of F actin assembly, and colchicine, a disrupting agent for tubulin, exert severe inhibitory effects on type I collagen induced superoxide formation. In contrast, the same cytochalasin B enhances the stimulation by the peptide fMet-Leu-Phe. The latter effect points out to the intervention of actin and tubulin in the reaction to type I collagen.

Inositol trisphosphate increases sharply after collagen stimulation, and calcium ion also increases for a short period of about 30 s. From these results, it is inferred that the activation of the type I collagen receptor is transmitted to a phospholipase C, which liberates inositol trisphosphate and diacylglycerol. Few studies have pointed to cascades of stimulations involving beta(2) integrins (28) . Inositol trisphosphate stimulates the output of calcium ions from the endoplasmic reticulum. Calcium signaling through Mac 1 has been described(29, 30) , in the case of cross-linking of this integrin by monoclonal antibodies. The stimulation depends on the presence of Ca in the medium surrounding cells. This requirement is at present unexplained. It may be related to the binding of collagen to the receptor. The effect of Ca on enzyme-containing granules probably depends on the actomyosin system responsible for the exocytosis of these granules. The effect of calcium on the activation of the NADPH-oxidase system of PMN is difficult to explain and may be due to a calcium-dependent isoform of protein kinase C able to phosphorylate the cytoplasmic protein p47, a preliminary step for the assembly of the NADPH-oxidase at the membrane and to its activation.

A role for diacylglycerol in the process of PMN stimulation with type I collagen by activating a protein kinase C was confirmed by the inhibiting effect exerted by staurosporine and calphostin C. Nevertheless, another inhibitor of protein kinase C, H-7, did not inhibit the process, whereas it inhibited the stimulation exerted by the peptide fMet-Leu-Phe. Collagen stimulates the translocation of protein kinase C to the plasma membrane, as demonstrated by measurements of changes in enzyme activity.

The alpha(L)beta(2) integrin, when liganded by type I collagen, is phosphorylated on tyrosyl residues as demonstrated by the use of monoclonal antibodies to phosphotyrosine reacting with the subunits of the integrin separated by PAGE. PMA or fMet-Leu-Phe treatments of monocytes induce the phosphorylation of CD18, mainly on seryl residues, and to a lesser extent on threonyl and tyrosyl residues(16, 31) . Phosphoserine was also detected on CD11a (16) . On which residues of the alpha(L) and beta(2) peptide chains does this reaction take place? The beta(2) chain contains 1 tyrosyl residue in its intracellular domain(32) . Four seryl residues but no tyrosyl are present in the intracellular domain of alpha(L). However, in the transmembrane domain, the 6th residue closer to the cytoplasmic domain is a tyrosine(23) . Our results suggest that it might be accessible to an intracellular tyrosine kinase. Tyrosine phosphorylation of several intracellular proteins is a major transduction pathway described for beta(1) integrins (33) . It also occurs by stimulating PMNs by fMet-Leu-Phe or TNFalpha(19, 34) . In this study, we show tyrosine phosphorylation of the two chains of an integrin upon its reaction with one of its ligands, opening new horizons on the way this integrin is able to transmit information to cytoplasm by binding specific proteins through SH(2) domains.

Polymorphonuclear neutrophils undergo multiple stimulations in order to cope with all the situations of defense of the organism against the many invader cells or toxic substances. Specific membrane receptors exist for every stimuli. At the present time, only a few steps of the transduction pathways for these messages are known and most of them concern the effect of the peptide fMet-Leu-Phe. In this paper, we describe a somewhat different system of signaling, depending on type I collagen or, more probably, on the large fragments of collagen that are liberated during the initial degradative steps of tissue inflammation or wound healing. The transduction system is characterized by several distinct features; the receptor is an integrin (namely alpha(L)beta(2)), the integrin is phosphorylated on tyrosine residues belonging to both subunits, there is no G protein involved, and cytoskeleton participates in the stimulation pathway, which involves inositol trisphosphate, calcium ion, and protein kinase C.


FOOTNOTES

*
This work was made possible by grants from CNRS (EP 89) and from the University of Reims (Mission de la Recherche, Ministère Enseignement Supérieur). The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore by hereby marked ``advertisement'' in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

§
To whom correspondence should be addressed: Laboratory of Biochemistry, Faculty of Medicine, CNRS EP 0089, University of Reims, 51 rue Cognacq Jay, F 51095 Reims Cedex, France.

(^1)
The abbreviations used are: PMN, polymorphonuclear neutrophil leukocyte(s); PAGE, polyacrylamide gel electrophoresis; Fmoc, 9-fluorenylmethylchloroformate; PMA, phorbol 12-myristate 13-acetate.


ACKNOWLEDGEMENTS

We express our thanks to C. Perreau for beautiful technical work, to Dr. G. Bellon for initiating the studies on the chromatographic fractionation of receptors, to Dr. L. Martiny for showing us the technique of purification of inositol phosphates, and to Dr. Legendre for improving the syntax of this paper.


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