©1995 by The American Society for Biochemistry and Molecular Biology, Inc.
Structural Features Mediating Fibrin Selectivity of Vampire Bat Plasminogen Activators (*)

(Received for publication, May 22, 1995; and in revised form, August 18, 1995)

Peter Bringmann (§) Daniel Gruber Alexandra Liese Luisella Toschi Jörn Krätzschmar Wolf-Dieter Schleuning Peter Donner

From the Research Laboratories of Schering AG Berlin, D-13342 Berlin, Federal Republic of Germany

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
ACKNOWLEDGEMENTS
REFERENCES

ABSTRACT

The distinguishing characteristic of vampire bat (Desmodus rotundus) salivary plasminogen activators (DSPAs) is their strict requirement for fibrin as a cofactor. DSPAs consist of structural modules known from urokinase (u-PA) and tissue-type plasminogen activator (t-PA) such as finger (F), epidermal growth factor (E), kringle (K), and protease (P), combining to four genetically and biochemically distinct isoenzymes, exhibiting the formulas FEKP (DSPAalpha1 and alpha2) and EKP and KP (DSPAbeta and DSPA). Only DSPAalpha1 and alpha2 bind to fibrin. All DSPAs are single-chain molecules, displaying substantial amidolytic activity. In a plasminogen activation assay, all four DSPAs are almost inactive in the absence of fibrin but strongly stimulated by fibrin addition. The catalytic efficiency (k/K) of DSPAalpha1 increases 10^5-fold, whereas the corresponding value of t-PA is only 550. The ratio of the bimolecular rate constants of plasminogen activation in the presence of fibrin versus fibrinogen (fibrin selectivity) of DSPAalpha1, alpha2, beta, , and t-PA was found to be 13,000, 6500, 250, 90, and 72, respectively. Whereas all DSPAs are therefore more fibrin dependent and fibrin selective than t-PA, the extent depends on the respective presence of the various domains. The introduction of a plasmin-sensitive cleavage site in a position akin to the one in t-PA partially obliterates fibrin cofactor requirement. Fibrin dependence and fibrin selectivity of DSPAs are accordingly mediated by fibrin binding, which involves the F domain, as yet undefined determinants within the K and P domains, and by the absence of a plasmin-sensitive activation site. These findings transcend the current understanding of fibrin-mediated stimulation of plasminogen activation: in addition to fibrin binding, specific protein-protein interactions come into play, which stabilize the enzyme in its active conformation.


INTRODUCTION

Plasminogen activators (PAs), (^1)such as t-PA and u-PA, are highly specific serine proteases, which catalyze the hydrolysis of the Arg-Val peptide bond of Glu-plasminogen. The activation product, plasmin, is a potent protease, which digests fibrin and several extracellular matrix proteins. Plasmin also processes the single-chain precursors of t-PA and u-PA to the more active two-chain forms. In contrast to u-PA, the rate of plasminogen activation by t-PA increases by 2-3 orders of magnitude in the presence of fibrin or fibrin(ogen) degradation products (Camiolo et al., 1971; Hoylaerts et al., 1982; Ranby, 1982; Bergum and Gardell, 1992). Both t-PA and its substrate, Glu-plasminogen, bind to fibrin, forming a ternary complex that facilitates the conversion of Glu-plasminogen (Hoylaerts et al., 1982; Ranby, 1982; Fears, 1989). t-PA consists of several structural motifs known by structural homology from other proteins: an N-terminal fibronectin-like finger (F), an epidermal growth factor (E), two kringles (K1 and K2), and a serine protease domain (P) (Pennica et al., 1983; Patthy, 1990). Several authors suggested the F domain and the lysine binding site (LBS) of the K2 domain to be the major contributors to t-PA fibrin affinity and to the observed fibrin-mediated enhancement of plasminogen activation (van Zonneveld et al., 1986; Verheijen et al., 1986; de Munk et al., 1989). Recent results, however, indicate that t-PA interacts with fibrin via a binding region that comprises surface areas of other structural modules as well, including the protease domain (Bennett et al., 1991).

In recent years, thrombolytic treatment with t-PA has emerged as state of the art therapy of acute myocardial infarction (Topol, 1991; Collen and Lijnen, 1991). However, when administered in therapeutic doses, t-PA, due to its limited fibrin selectivity, causes plasminemia that may contribute to bleeding complications (Rao et al., 1988; Arnold et al., 1989). Therefore, considerable efforts have been devoted to the design of new variants of t-PA exhibiting improved fibrin selectivity (Higgins and Bennett, 1990; Lijnen and Collen, 1991). Recently, a novel mutein of t-PA called TNK, which is more fibrin selective than t-PA, has been characterized (Keyt et al., 1994; Collen et al., 1994).

We and others (Gardell et al., 1989; Krätzschmar et al., 1991) have previously reported the cloning, expression, and characterization of plasminogen activators derived from the saliva of vampire bats. A total of four different Desmodus rotundus salivary plasminogen activators (DSPAs), which we named DSPAalpha1, alpha2, beta, and have been cloned, expressed, and characterized. DSPAalpha1 and alpha2 encompass an F, E, K, and P domain, while DSPAbeta lacks the finger module and DSPA contains only a K and a P domain. Apart from these differences, DSPAs are very similar (88.7-99.5% amino acid sequence identity; Krätzschmar et al.(1991)). The amino acid sequence of human t-PA is similarly related (72.3% (DSPAalpha1) and 74.2% (DSPAalpha2) identity; Krätzschmar et al.(1991)). Like u-PA, all DSPAs only contain a single K domain rather than two, as is the case for t-PA. The K module of DSPAs is more similar to the K1 domain of t-PA and does not exhibit an LBS. Furthermore, a plasmin-sensitive activation site, present in the N-terminal region of the t-PA protease domain is absent in DSPAs. Therefore, DSPAs activate plasminogen as single chain molecules (Gardell et al., 1989; Krätzschmar et al., 1991).

Functionally, DSPAs differ from t-PA by their strict requirement for a fibrin cofactor. This was studied in great detail for Bat-PA (equivalent to DSPAalpha2) by Bergum and Gardell(1992) and has been reported for DSPAalpha1 as well (Schleuning et al., 1992). When compared to t-PA, Bat-PA and DSPAalpha1 demonstrated an equal or even higher thrombolytic potency in several animal models of arterial thrombosis (Gardell et al., 1991; Mellot et al., 1992; Witt et al., 1992, 1994; Muschick et al., 1993). Importantly, while being equally effective as t-PA, fibrinogen degradation or alpha2-antiplasmin consumption were considerably lower with Bat-PA and DSPAalpha1 (Gardell et al., 1991; Mellot et al., 1992; Witt et al., 1992; Muschick et al., 1993).

The present study evaluates the fibrin selectivities of the recombinant forms of all naturally occurring DSPAs and compares these data with those obtained for t-PA. Furthermore, we present data that suggest a molecular mechanism for the unique fibrin selectivity of DSPAs.


MATERIALS AND METHODS

Mutagenesis

Oligonucleotide-directed mutagenesis was performed as described by Lewis and Thompson(1990) using the Promega mutagenesis kit. DSPAalpha1 cDNA (Krätzschmar et al., 1991) was subcloned into the EcoRI-HindIII sites of the pSELECT-1 phagemid polylinker. The plasmin-sensitive site was introduced annealing the following oligonucleotide: 5`-CAGCCTCGCATTAAAGGAGGACTC-3`. T-PA cDNA (Waller and Schleuning, 1985) was ligated into the HindIII site of the same vector. The plasmin-sensitive site was inactivated by hybridizing the following oligonucleotide: 5`-CCTCAGTTTCACAGCACAGGAGGGCTC-3`. Sequence alterations were verified by DNA sequencing (Sanger et al., 1977).

Purified Proteins and Substrates

Recombinant DSPAs were produced in BHK cells transfected with pMPSVEH expression vectors (Artelt et al., 1988; Wirth et al., 1991) harboring the cDNAs encoding wild-type DSPAs alpha1, alpha2, beta, and (Krätzschmar et al., 1991), the mutated DSPAalpha1 cDNA, or the mutated t-PA cDNA (Krätzschmar et al., 1992). The secreted recombinant plasminogen activators were purified from cell culture supernatants by affinity chromatography on immobilized Erythrina trypsin inhibitor (Heussen et al., 1984), which was purchased from Erytech Services (PTY Ltd., Arcadia, South Africa). Recombinant t-PA (Actilyse®) was obtained from Dr. Karl Thomae (GmbH, Biberach, Germany). Human Glu-plasminogen, received from Chromogenix (Sweden), was liberated from contaminating lysine by gel filtration using PD-10 columns. Plasminogen-free human fibrinogen was purchased from Calbiochem, and human thrombin was ordered from Sigma. The chromogenic substrates S-2765 (N-alpha-Cbo-D-Arg-Gly-Arg-p-nitroanilide-dihydrochloride) and FlavigenPli (D-But-CHT-Lysp-nitroanilide-dihydrochloride) were obtained from Chromogenix and Biopool, respectively. The two-chain form of the mutein [H189R,S190I,T191K] DSPAalpha1 and of t-PA was prepared by treatment with plasmin immobilized to Sepharose according to Higgins and Vehar(1987). Protein concentrations were determined spectrophotometrically at 280 nm, using extinction coefficients (cm/mg) for 1 mg/ml solutions at 280 nm of 1.70 and 1.62 for Glu-plasminogen (Robbins and Summaria, 1970) and fibrinogen (Blombäck, 1958), respectively. The extinction coeffients of 1.71, 1.65, 1.69, 1.68, and 1.81 for DSPAalpha1, DSPAalpha2, DSPAbeta, DSPA, and t-PA, respectively, were calculated employing the program PeptideSort of the Wisconsin Sequence Analysis Package (Devereux et al., 1984). The integrity of Glu-plasminogen was verified by N-terminal sequence analysis.

Radioiodination of PAs

The DSPA variants were labeled by the iodogen method according to the manufacturer's protocol (Pierce, no. 28600) and exhibited specific activities of 40-80 KBq/µg protein. In brief, DSPAs (0.2 mg/ml) were labeled with [I]iodine in 50 mM HEPES, pH 7.5, 0.1 M NaCl in iodogen-coated tubes containing 3.7 MBq sodium [I]iodide. Following incubation for 15 min at 4 °C, the reactants were separated by gel filtration using a PD-10 column (Pharmacia Biotech Inc.). Protein concentration of labeled DSPAs was determined by a microtiter plate version of the method described by Bearden(1978).

Fibrin Binding

The binding of DSPAs to forming fibrin clots was studied as a competition assay using a slightly modified version of the method described by Rijken et al. (1982). In brief, human fibrinogen (plasminogen-free) (120 µg/ml (294 nM clottable protein), final concentration) was mixed with a constant amount of I-labeled DSPAs (5-10 nM, approximately 130,000 cpm), various amounts of unlabeled DSPAs (0-5 µM, final concentration), and human thrombin (0.1 NIH units/ml, final concentration). The total volume was 0.1 ml, and the buffer was composed of 25 mM Tris, 40 mM NaCl, 0.5 mM CaCl(2), pH 8.0, containing 0.01% Tween 20. The mixture was incubated for 1 h at 37 °C, and the clots were compacted by centrifugation in a Heraeus Biofuge 15 at 15,000 rpm for 15 min. Unbound PA was directly quantified by counting of an aliquot of the supernatant in a Canberra Packard Cobra II counter. The amount of specifically bound DSPA was calculated as the difference between the total amount of DSPA and that determined in the supernatant following background correction of nonspecific binding (maximum 4% of total cpm).

The dissociation constant for the binding of DSPAs to fibrin and the numbers of binding sites were calculated by nonlinear regression analysis of the data according to the Scatchard equation employing the programs EBDA (equilibrium binding data analysis) and LIGAND, originally written by Munson and Rodbard(1980) and modified by G. A. McPherson (V 2.0), which were obtained from Elsevier-Biosoft (Cambridge, United Kingdom).

Kinetics of Plasminogen Activation

All kinetics were measured spectrophotometrically at ambient temperature using a Bio-Rad microplate reader (model 3550) that was coupled to a Macintosh IIci. Kinetics of plasminogen activation were performed using the coupled enzymatic assay outlined by Nieuwenhuizen et al. (1985) with slight modifications. Briefly, individual assay samples encompassed the following ingredients: 0.5 nM plasminogen activator, 100 µg/ml fibrin(ogen) where stated (0.13 units/ml of human thrombin in case of fibrin), 0.05-8 µM Glu-plasminogen, and 1 mM FlavigenPli in a total volume of 0.15 ml of PCLA buffer (Jones and Meunier, 1990). When plasminogen activation was analyzed in the presence of -amino caproic acid (EACA), individual assays contained 20 mM EACA and, for some assays, in addition 100 µg/ml fibrin. All assays were done in triplicates for each plasminogen concentration and were repeated at least 3-fold. To correct for turbidity due to the presence of fibrin, DeltaA - A/min was monitored. Although FlavigenPli hydrolysis by thrombin was not significant and there was no detectable autohydrolysis, a blank (without plasminogen activator) was determined for each plasminogen concentration in duplicate. This control value was subtracted, and the resulting value was converted to [pNA] using appropriate standard curves. The acceleration of pNA generation (d^2[pNA]*dt), which is directly proportional to the velocity of plasminogen activation, was determined by nonlinear regression analysis of 2nd order polynomial plots of [pNA] versus time. It was then plotted against the concentration of plasminogen, and kinetic parameters k, K(m), and k/K(m) were calculated by nonlinear regression of data points according to the Michaelis-Menten equation. Computing was carried out on a Macintosh IIci using Kaleidagraph and Microplate Manager software. Kinetic constants of FlavigenPli hydrolysis by plasmin were determined under the aforementioned conditions and verified the assumption that K(m)(pli) [FlavigenPli] (Drapier et al., 1979) (data not shown).

Kinetics of S-2765 Hydrolysis

Kinetics of S-2765 hydrolysis were performed similarly. Assay volume was 0.15 ml containing 10 nM plasminogen activator, 100 µg/ml fibrin(ogen), and 0.02-4 mM S-2765 in PCLA buffer. Individual assays performed as triplicates were repeated at least three times. Hydrolysis of S-2765 by thrombin was not detectable under these conditions. Omitting the plasminogen activator, blanks carried out in duplicates were determined for every concentration of S-2765. As described above, DeltaA - A/min was calculated and converted to [pNA]. In this case velocities, calculated from linear plots of [pNA] versus t, were plotted versus concentration of S-2765 and analyzed by nonlinear regression to obtain kinetic parameters K(m) and k.


RESULTS

DSPAs alpha1, alpha2, beta, and were expressed in BHK cells as described (Krätzschmar et al., 1992). Recombinant proteins were purified to homogeneity from cell culture supernatants by affinity chromatography on immobilized Erythrina trypsin inhibitor (Heussen et al., 1984). As judged from SDS-PAGE analysis, preparations of recombinant DSPAs alpha1, alpha2, beta, and were homogeneous, and the proteins displayed an apparent molecular mass of 52, 52, 46, and 44 kDa, respectively (Fig. 1, lanes 1-4).


Figure 1: SDS-PAGE of purified recombinant DSPAs and t-PA. Prior to electrophoresis on a SDS-gel containing 12.5% polyacrylamide (Laemmli 1970), all samples were reduced by the addition of dithiothreitol (12.5 mM). Approximately 3 µg of each protein was loaded. The gel was stained with Coomassie Brilliant Blue (G250). Proteins were produced as outlined under ``Materials and Methods.'' Lane 1, rDSPAalpha1; lane 2, rDSPAalpha2; lane 3, rDSPAbeta; lane 4, rDSPA; lane 5, marker proteins (M) whose molecular mass is indicated on the right; lane 6, rt-PA (Actilyse®); lane 7, [R275H,I276S,K277T] t-PA lacking the plasmin-sensitive site; lane 8, [H189R,S190I,T191K] DSPAalpha1 containing a plasmin-sensitive site.



DSPA Affinity for Fibrin

Investigating the fibrin affinity of DSPAs isolated from bat saliva, we had previously observed that only the two full-length variants, DSPAalpha1 and alpha2, exhibited affinity to fibrin, whereas DSPAs beta and did not (Schleuning et al., 1992). Using I-iodinated recombinant DSPAs, we assessed their affinity for forming fibrin clots in vitro. Binding of both DSPAs alpha1 and alpha2 was saturable and exhibited similar characteristics (Fig. 2). A Scatchard analysis of the interaction between forming fibrin clots and DSPAalpha1 or alpha2 revealed virtually identical K(d) values of 154 ± 43 nM and 131 ± 15 nM, and similar molar binding ratios of 0.48 ± 0.08 and 0.61 ± 0.14, respectively (Fig. 2). Interaction with fibrin does not involve a lysine binding site because it was not impaired by the presence of lysine or EACA even in a molar excess of several orders of magnitude (data not shown). Using the protocol outlined under ``Materials and Methods,'' we were unable to detect measurable binding to fibrin of DSPAs beta and (data not shown).


Figure 2: Scatchard analysis of the interaction between DSPAalpha1 or DSPAalpha2 and forming fibrin clots. A, Scatchard analysis of fibrin binding data obtained for I-DSPAalpha1. The plot is based on a model involving one type of binding site. Inset, equilibrium binding of I-DSPAalpha1 to fibrin. Binding was determined at variable concentrations of unlabeled DSPAalpha1 as described under ``Materials and Methods.'' Each point is represented by the results of three independent determinations. The average standard error for the equilibrium binding curve was approximately 7%. Specific binding was calculated by subtracting nonspecific binding (e.g. in the presence of excess unlabeled DSPAalpha1) from total binding. Nonspecific binding was 4% of total cpm. B, Scatchard plot of fibrin binding data of I-DSPAalpha2. The plot is based on a model involving a sole type of binding site. Inset, equilibrium binding of I-DSPAalpha2 to fibrin. Binding was determined as described under ``Materials and Methods.'' The results of three independent experiments are displayed. The average standard error for the equilibrium binding curve was about 6%. Specific binding was calculated by subtracting nonspecific binding (e.g. in the presence of excess unlabeled DSPAalpha2) from total binding. Nonspecific binding was 6% of total cpm.



Glu-Plasminogen Activation by DSPAs and by t-PA in the Absence and Presence of a Fibrin(ogen) Cofactor

In the absence of a fibrin(ogen) cofactor, DSPAs alpha1, alpha2, beta, and exhibited similar, but very low bimolecular rate constants ranging from 4.4 to 9.8 M s (Table 1). The corresponding K(m) values were approximately 10 µM or higher, and their k values were in the range of 1.0 * 10 s, indicating that DSPAs hardly showed affinity for the substrate and were virtually unable to activate Glu-plasminogen.



In the presence of fibrin, however, the catalytic efficiency of DSPAs was augmented by several orders of magnitude. The steepest increase by a factor of 10^5, resulting in a k/K(m) value of 684,000 M s, was observed for DSPAalpha1. The bimolecular rate constant of DSPAalpha2 was raised to 517,000 M s, corresponding to a 53,000-fold enhancement (Table 1). DSPAs beta and exhibited considerably smaller catalytic efficiencies of 9900 M s and 3510 M s, reflecting a 1650- and 800-fold increase in catalytic activity, respectively. This demonstrates that binding of the DSPAs to fibrin significantly contributes to enhanced plasminogen activation. For DSPAalpha1 and alpha2, the fibrin-mediated enhancement of catalytic efficiency resulted from both a moderate decrease (25- and 34-fold) in K(m) and a concomitant profound increase (4300- and 1550-fold) in k, respectively. Interestingly, despite their high degree of homology (89% identity in amino acid sequence) (Krätzschmar et al., 1991), the unstimulated activity of DSPAalpha2 was slightly higher than that of DSPAalpha1, which, however, was more active in the presence of fibrin (Table 1). The 2-fold higher fibrin-mediated enhancement of the catalytic efficiency of DSPAalpha1 was due to a steeper increment in the k value of DSPAalpha1 rather than a more pronounced decrease in its K(m) (Table 1). The reduction in K(m) and in particular the increase in k was significantly smaller for DSPAs beta and (Table 1).

In comparison to the absence of a cofactor, fibrinogen promoted the catalytic efficiency of DSPAs by 7-9-fold, resulting in k/K(m) values ranging from 39 to 79 M s, which were several orders of magnitude smaller than those observed in the presence of fibrin (Table 1). The ratio of catalytic efficiencies in the presence of fibrin to the corresponding values in the presence of fibrinogen, which serves as a measure of ``fibrin selectivity'', amounted to 12,900 for DSPAalpha1. The bimolecular rate constant of DSPAalpha2 in the presence of fibrin was 6550-fold higher than that in the presence of fibrinogen. The respective values for DSPAs beta and were 235 and 90 (Table 1). DSPAalpha1 therefore exhibited the highest fibrin selectivity, and this was mainly attributable to its superior stimulation by fibrin.

The data summarized in Table 1also depict how the kinetic parameters of DSPAs compare to those obtained for t-PA. In the absence of a fibrin(ogen) cofactor, t-PA was 260-fold more efficient in activating Glu-plasminogen than DSPAalpha1. In the presence of fibrin, however, both plasminogen activators were similarly effective (Table 1). The enhancement of the bimolecular rate constant of t-PA in the presence of fibrin was only 550-fold as compared to 10^5-fold for DSPAalpha1. In the presence of fibrinogen, the catalytic efficiency of t-PA was increased to 13,600 M s, which was 260- and 170-fold higher than the respective values measured for DSPAalpha1 and alpha2 (Table 1). Fibrin increased the catalytic efficiency of t-PA by only 72-fold over that in the presence of fibrinogen, meaning that DSPAalpha1 was about 180-fold more fibrin selective than t-PA. DSPAalpha2 exhibited a 90-fold higher fibrin selectivity than t-PA, and even the finger-deficient variant DSPAbeta was still 3-fold more fibrin selective. The latter strongly indicates that fibrin selectivity is not merely a consequence of the plasminogen activator's affinity for fibrin.

Fibrin Stimulation and Fibrin Selectivity Depend on the Presence of a Plasmin-sensitive Site

Several studies indicated that the abolition of the t-PA plasmin-sensitive site led to an improved fibrin selectivity of the t-PA molecule, which was mainly due to a reduced activity in the absence of a stimulator (Petersen et al., 1988; Boose et al., 1989; Higgins et al., 1990; Paoni et al., 1993). Since the protease domains of DSPAs do not contain a plasmin-sensitive cleavage site, we wanted to estimate the contribution to fibrin stimulation and selectivity of this structurally distinct feature. To allow for a direct comparison in our experimental systems, cDNAs encoding plasmin-sensitive DSPAalpha1 ([H189R,S190I,T191K] DSPAalpha1) as well as plasmin-insensitive sct-PA ([R275H,I276S,K277T] t-PA) were constructed and expressed as outlined under ``Materials and Methods.'' Homogeneity of affinity-purified muteins was verified by SDS-PAGE (lanes 6-8, Fig. 1). Similar to t-PA, the preparation of [H189R,S190I,T191K] DSPAalpha1 contained about 10% two-chain material (lanes 6 and 8, Fig. 1) as verified by Western analysis (data not shown). Whereas the DSPAalpha1 mutein was easily converted to its two-chain form by treatment with plasmin, [R275H,I276S,K277T] t-PA remained single chain (Fig. 3).


Figure 3: Plasmin-mediated conversion of [R275H,I276S,K277T] t-PA and [H189R,S190I,T191K] DSPAalpha1. Recombinant proteins were prepared as described under ``Materials and Methods.'' Approximately 5 µg each of t-PA, [R275H,I276S,K277T] t-PA, and [H189R,S190I,T191K] DSPAalpha1 were incubated for 30 min at 37 °C in the absence (lanes 2, 4, and 6) or presence of Sepharose-immobilized plasmin (lanes 3, 5, and 7). The samples were analyzed by SDS-PAGE as outlined in the legend to Fig. 2. Lane 1, marker proteins (M) whose molecular mass is indicated on the left; Lanes 2, 4, and 6, t-PA, [R275H,I276S,K277T] t-PA, and [H189R,S190I,T191K] DSPAalpha1, respectively, incubated in the absence of plasmin, or as shown in lanes 3, 5, and 7, treated with plasmin.



In the absence of a stimulator, the DSPAalpha1 mutein exhibited a bimolecular rate constant of 135 M s, which reflected a 20-fold increase over that of wild-type DSPAalpha1. The catalytic efficiency of sct-PA was reduced, in comparison to t-PA, by 50-fold to 34 M s (Table 1), which is in good agreement to the activity decrease observed previously (Andreasen et al., 1991; Petersen et al., 1988; Tate et al., 1987). Fibrinogen raised the k/K(m) value of plasmin-sensitive DSPAalpha1 mutein to 516 M s, which in comparison to the wild type, corresponded to a 10-fold increase. The respective value (638 M s) of sct-PA was 20-fold decreased. In the presence of fibrin, however, both muteins displayed catalytic efficiencies (DSPAalpha1 mutein, 565,000 M s, and t-PA mutein, 525,000 M s) that were similar to the respective wild-type proteins (Table 1). In comparison to fibrinogen, fibrin promoted the catalytic efficiency of plasmin-sensitive DSPAalpha1 by 1100-fold, which was 12-fold less than that of the uncleavable wild-type enzyme. In case of t-PA, the absence of the cleavage site resulted in an 11-fold increase of its fibrin selectivity. Importantly, DSPAalpha1 and DSPAalpha2 were still about 16- and 8-fold more fibrin selective than uncleavable sct-PA, and plasmin-sensitive DSPAalpha1 was 15-fold more fibrin selective than t-PA (Table 1), implying that other features apart from the lack of the plasmin-sensitive cleavage site must contribute to the superior fibrin selectivity of DSPAs.

Hydrolysis of S-2765 by DSPAs and t-PA in the Presence and Absence of Fibrin or Fibrinogen

The contribution to fibrin stimulation of the direct interaction between the plasminogen activators and fibrin was assessed by monitoring PA-catalyzed hydrolysis of S-2765, a small chromogenic substrate, in the absence or presence of a fibrin cofactor. Fibrin increased the k/K(m) of DSPAalpha1 and alpha2 equally by about 14-fold over that in its absence, while fibrinogen led only to a marginal enhancement of less than 2-fold (Table 2). The fibrin-mediated promotion of their bimolecular rate constant was due to a 5-fold drop in K(m) and a 2-3-fold increase in k. Although fibrin and fibrinogen exerted quantitatively similar effects, their absolute catalytic efficiency of S-2765 hydrolysis was different. Independent of the presence or absence of a fibrin cofactor, DSPAalpha2 was always 2-fold more efficient in hydrolyzing S2765 than DSPAalpha1. This elevated activity was brought about by a higher k value. As expected, because they do not bind to fibrin, an appreciable fibrin-mediated enhancement of S-2765 hydrolysis by DSPAs beta and did not occur (Table 2).



In the absence of a fibrin(ogen) cofactor, DSPAalpha1 and -alpha2 exhibited 17 and 37.5%, respectively, of t-PA catalytic efficiency. While fibrinogen had only a very small effect on the k/K(m) of t-PA, fibrin promoted its bimolecular rate constant by 4-fold. In the presence of the latter the activity of DSPAalpha2 was equivalent to that of t-PA, whereas S-2765 hydrolysis by DSPAalpha1 was 2-fold less efficient (Table 2).

As observed for t-PA and DSPAalpha1, the extent of fibrin-mediated stimulation of S-2765 hydrolysis was dependent on whether they occurred in their single or two-chain forms. The single chain forms of DSPAalpha1 and t-PA were more highly stimulated than their two-chain counterparts (Table 2). The intrinsic activity of tct-PA was not significantly stimulated by fibrin, while tc DSPAalpha1's catalytic efficiency was still enhanced (2.6-fold), albeit 5-fold less than that of the single chain molecule. This effect was attributed to an increased k, which was not observed for t-PA. By comparison to the wild-type molecule, the tc DSPAalpha1 mutein exhibited a 4-fold higher catalytic efficiency in the absence of a fibrin(ogen) cofactor (Table 2).

Influence of EACA on Plasminogen Activation by DSPAs and t-PA

The influence of plasminogen conformation on the stimulation of plasminogen activation by DSPAs and t-PA was addressed using EACA. Upon occupying plasminogen's LBS, EACA mediates the conversion of plasminogen's compact structure into a more extended and open form (Mangel et al., 1990; Ponting et al., 1992). Since plasminogen binds to fibrin via its LBS, it is thought that the flexible conformation of the EACA-complexed protein mimics that of fibrin-bound plasminogen. In the presence of EACA, conversion of plasminogen by all plasminogen activators tested was enhanced by 4-9-fold (Table 3), in line with results published previously for t-PA (Urano et al., 1988). Since EACA did not influence the rate of FlavigenPli hydrolysis by plasmin (data not shown), the increase in the bimolecular rate constant was most likely due to a change in plasminogen conformation, rendering it a more favorable substrate.



Since alterations in plasminogen conformation only accounted for a small portion of fibrin's stimulatory effect, it is evident that the major contribution to fibrin stimulation is mediated by the ternary complex formation and/or the interaction of DSPAalpha1 and alpha2 with fibrin (Hoylaerts et al., 1982; Wu et al., 1990). To discriminate between these two mechanisms, we have measured enzyme kinetics in the presence of both fibrin and EACA. Under these conditions, only the plasminogen activator is able to bind to fibrin, whereas binding of plasminogen to fibrin is inhibited (Lucas et al., 1983; Nesheim et al., 1990). Binding of t-PA is solely mediated by the finger domain because kringle 2-dependent binding of t-PA to fibrin is inhibited (van Zonneveld et al., 1986; Nesheim et al., 1990).

By comparison to their catalytic efficiencies in the presence of fibrin alone, the additional presence of EACA diminished the catalytic activities of DSPAs alpha1, alpha2, tc DSPAalpha1, and t-PA by 90-24-fold (Table 4). As expected, this decrease was entirely due to an increase in the apparent K(m), since the k values were similar to that obtained in the presence of fibrin alone ( Table 1and Table 4). Hence, the dissociation of plasminogen from the fibrin template caused similar decrements, within the same order of magnitude, of plasminogen activator catalytic efficiencies. However, a comparison of the bimolecular rate constants in the presence of fibrin and EACA to those in the presence of EACA alone revealed striking differences between DSPAs and t-PA. The addition of fibrin to the reaction mixture that already contained EACA raised DSPAalpha1's k/K(m) from 26 to 7790 M s (about 300-fold), whereas that of t-PA was promoted by only 6-fold from 7480 to 41,270 M s ( Table 3and Table 4). In accordance with our earlier observation, the activity of DSPAalpha1 was 2-fold more highly promoted by the addition of fibrin than that of DSPAalpha2 (Table 4). In the presence of fibrin and EACA, the catalytic efficiency of the plasmin-sensitive DSPAalpha1 mutein was enhanced to 11,020 M s, which represented an only 12-fold increase over that, 890 M s, in the presence of EACA alone.




DISCUSSION

There are three plausible mechanisms pertinent to fibrin-mediated stimulation of plasminogen activation, all based on protein-protein interactions: 1) a template-mediated rendezvous mechanism furthering the physical encounter of both enzyme and substrate, 2) the exposure of the activation site of plasminogen, following a conformational change induced by fibrin binding, and (3) a stabilizing effect of fibrin on the active site of plasminogen activators, probably mediated by domain-domain interactions.

We have attempted to attribute the observed stimulatory effects to one or the other of these mechanisms. In contrast to t-PA, the major contribution of fibrin to its overall stimulatory effect on plasminogen conversion by DSPAs alpha1 and alpha2 is mediated by its interaction with the plasminogen activator itself (Table 4). The template effect appears to be less important, whereas it is paramount to fibrin-mediated enhancement of plasminogen activation by t-PA (Hoylaerts et al., 1982). Corroborating the results from direct measurements of fibrin binding, an interaction of DSPAalpha1 or alpha2 and fibrin is also demonstrated by the enhancement of S-2765 hydrolysis. Upon binding to fibrin, the catalytic activities of DSPAalpha1 and alpha2 were raised by about 1 order of magnitude, whereas those of DSPAs beta and were increased only marginally (Table 2). Therefore, in case of DSPAbeta and , the increase in the plasminogen activation rate is most likely due to a conformational change in plasminogen induced by its interaction with partially degraded fibrin (Suenson et al., 1984), although domain-domain interactions occurring within the DSPA molecules might also be involved.

The striking difference between DSPAs and t-PA, as far as fibrin stimulation is concerned, is not a consequence of disparate fibrin affinities. The K(d) values of DSPAalpha1 and DSPAalpha2 (Fig. 2) are within the range of values published for t-PA (0.13-0.58 µM) (Higgins and Vehar, 1987; Husain et al., 1989; Nesheim et al., 1990; Bergum and Gardell, 1992; Horrevoets et al., 1994). The data are particularly consistent, if only finger-dependent binding of t-PA is analyzed. Under these conditions, Nesheim et al.(1990) measured a K(d) of 0.13 µM and a molar binding ration of 0.6, values that are almost identical to those of DSPAalpha1 and alpha2 (Fig. 2). Furthermore, the dependence on the fibrin concentration was very similar for DSPAs and t-PA. Half-maximal velocities were achieved at 25 ± 3, 31 ± 5, and 13 ± 2 µg/ml for DSPAalpha1, DSPAalpha2, and t-PA, respectively (data not shown).

All DSPAs exhibited only marginal activity in the absence of a fibrin(ogen) cofactor (Table 1). Upon addition of fibrinogen, their second order rate constants increased similarly by roughly 1 order of magnitude, which is in contrast to the markedly diverging stimulatory effect mediated by fibrin. For instance, in case of DSPAalpha1 and DSPAbeta, the extent of fibrin stimulation differs by a factor of 62 (Table 1). These data therefore suggest that the stimulatory effect exerted by fibrinogen is not conferred via the DSPAs but is rather mediated by an interaction between plasminogen and fibrinogen (Lucas et al., 1983).

The ratio of the bimolecular rate constants of plasminogen activation in the presence of fibrin versus fibrinogen is defined as fibrin selectivity. Since DSPAalpha1, alpha2, and t-PA exhibited very similar bimolecular rate constants in the presence of fibrin, the significant difference in fibrin selectivity of DSPAalpha1/alpha2 and t-PA is mainly caused by their unequal catalytic efficiencies in the presence of fibrinogen (Table 1).

To further understand the underlying structure-function relationship, we have analyzed the properties of a mutein of DSPAalpha1, whose protease domain contained a plasmin-sensitive site (Table 1Table 2Table 3Table 4). In the presence of fibrin, the catalytic efficiency of plasmin-sensitive DSPAalpha1 was strikingly less (24-fold) increased than that of the wild-type protein (Table 1). This decrease in fibrin stimulation was entirely attributable to a diminished stimulation via the plasminogen activator protease domain because upon prevention of the template effect by addition of -amino caproic acid, fibrin stimulated the catalytic efficiency only 12-fold as opposed to 300-fold as observed for DSPAalpha1 (Table 4). Since the bimolecular rate constants of DSPAalpha1 and its plasmin-sensitive mutein were almost identical in the presence of fibrin (Table 1), the decreased stimulatory effect was a consequence of the mutein's higher basal activity. Further, the fibrin selectivity of cleavable DSPAalpha1 was decreased about 12-fold (Table 1) and the fibrin-stimulated intrinsic catalytic activity about 5-fold (Table 2). Hence, the lack of a plasmin-sensitive site within the DSPAalpha1 protease domain contributes significantly to both the impressive stimulation by fibrin and its fibrin selectivity. Abolition of the plasmin-sensitive site of t-PA brings a quantitatively similar effect into bearing, namely a 28-fold increase in fibrin stimulation (Table 1). Concomitantly, the fibrin selectivity is improved 11-fold, again quantitatively equal to the effect observed for the cleavable DSPAalpha1 mutein. The role of the t-PA plasmin cleavage site for fibrin stimulation has been investigated previously, and similar results have been obtained (Tate et al., 1987; Petersen et al., 1988; Higgins et al., 1990). Nienaber et al.(1992) suggest that the interaction of the single-chain form of t-PA with fibrin(ogen) induces a conformational change at the active site stabilizing an ``active locked'' conformation. Since the influence on fibrin stimulation and on fibrin selectivity of a plasmin-sensitive site in the protease domain of DSPAalpha1 or t-PA is almost identical, it is likely that the stimulation of the DSPAalpha1 protease domain by fibrin is due to a similar mechanism.

Notably, plasmin-sensitive DSPAalpha1 was still 15-fold more fibrin selective than t-PA, and DSPAalpha1 discriminated more than 7-fold better between fibrin and fibrinogen than sct-PA (Table 1). This difference is also corroborated by amidolytic data. While fibrin raised the intrinsic catalytic activity of tc DSPAalpha1 by 2-3-fold over that in the presence of fibrinogen, the k/K(m) of tct-PA remained essentially unchanged (Table 2). Therefore, the heterotropic effect conferred by fibrin does not depend solely on the lack of the plasmin-sensitive cleavage site but involves other, yet unknown, determinants within the molecule.

Only DSPAalpha2 (Bat-PA) and t-PA have been evaluated in a way comparable to this study by other authors. Pertaining to t-PA, our data are similar to those previously reported (Rånby, 1982; Urano et al., 1988; de Vries et al., 1991; Bergum and Gardell, 1992). Our values were generally higher than those published for Bat-PA (corresponding to DSPAalpha2) by Bergum and Gardell(1992). This difference can be explained by use of different k values for plasmin-mediated hydrolysis of the chromogenic substrate (FlavigenPli versus SpectrozymePl). The relative stimulation factors, however, are in good agreement (the Bat-PA k/K(m) 43500-fold increase in the presence of fibrin, DSPAalpha2 52,700-fold). Fibrin (fibrin II) stimulated DSPAalpha2 catalytic efficiency 10,900-fold more than fibrinogen as compared to the ratio of 6550 determined in our system. Our data, however, do not confirm that in the absence of a stimulator the Bat-PA K(m) was 0.6 µM and therefore smaller than in the presence of fibrinogen (Bergum and Gardell, 1992). By contrast, DSPAalpha2 affinity for Glu-plasminogen was very low as indicated by a K(m) of 12.3 µM, a value very similar to those determined for DSPAalpha1 (9.5 µM) and sct-PA (17.7 µM). Also, our unstimulated K(m) value for t-PA, 5.2 µM, was similar to the 6.7 µM reported by Bergum and Gardell(1992) and agreed very well with the values of 7.6 and 9 µM published by Rånby(1982) and Urano et al.(1988), respectively.

In summary, we have provided a biochemical rationale for the striking fibrin selectivity of DSPAs: finger-dependent fibrin binding confers a heterotropic effect, which is conceivably mediated by domain-domain interactions on the protease domain to stabilize a preformed active site. Introduction of a plasmin-sensitive cleavage site partially obliterates the requirement for the fibrin cofactor. Further understanding of the molecular details of this interaction will depend on the results of structural analysis, which is currently underway.


FOOTNOTES

*
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. Tel.: 49-30-468-2130; Fax: 49-30-4691-6707.

(^1)
The abbreviations used are: PA, plasminogen activator; EACA, -amino caproic acid; PAGE, polyacrylamide gel electrophoresis; DSPA, D. rotundus salivary plasminogen activator; LBS, lysine binding site; pNA, p-nitroaniline; tcDSPAalpha1, two-chain DSPAalpha1; tct-PA, two-chain t-PA.


ACKNOWLEDGEMENTS

We are grateful to Drs. Michael McCaman, Linda Cashion, and Thomas Petri for fermentation of recombinant cell cultures. We thank Gisela Hübner-Kosney, Dyana Schwerdt, Dania Schmidt, and Andrea Toben for excellent technical support. We thank Dr. J. Verheijen for critical reading of the manuscript.


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