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Metabolic Mapping of Proteinase Activity with Emphasis on In Situ Zymography of Gelatinases : Review and Protocols

Wilma M. Frederiks and Olaf R.F. Mook

Academic Medical Center, University of Amsterdam, Department of Cell Biology and Histology, Amsterdam, The Netherlands

Correspondence to: Dr. Wilma M. Frederiks, Dept. of Cell Biology and Histology, Academic Medical Center, Meibergdreef 15, 1105 AZ Amsterdam, The Netherlands. E-mail: w.m.frederiks{at}amc.uva.nl

	Summary

Top Summary Introduction Metabolic Mapping of Protease... Zymography In Situ Zymography of... In Situ Zymography with... In Situ Zymography with... Literature Cited

 
Proteases are essential for protein catabolism, regulation of a wide range of biological processes, and in the pathogenesis of many diseases. Several techniques are available to localize activity of proteases in tissue sections or cell preparations. For localization of the activity of matrix metalloproteinases, in situ zymography was introduced some decades ago. The procedure is based on zymography using SDS polyacrylamide gels containing gelatin, casein, or fibrin as substrate. For in situ zymography, either a photographic emulsion containing gelatin or a fluorescence-labeled proteinaceous macromolecular substrate is brought into contact with a tissue section or cell preparation. After incubation, enzymatic activity is revealed as white spots in a dark background or as black spots in a fluorescent background. However, this approach does not allow precise localization of proteinase activity because of limited sensitivity. A major improvement in sensitivity was achieved with the introduction of dye-quenched (DQ-)gelatin, which is gelatin that is heavily labeled with FITC molecules so that its fluorescence is quenched. After cleavage of DQ-gelatin by gelatinolytic activity, fluorescent peptides are produced that are visible against a weakly fluorescent background. The incubation with DQ-gelatin can be combined with simultaneous immunohistochemical detection of a protein on the same section. To draw valid conclusions from the findings with in situ zymography, specific inhibitors need to be used and the technique has to be combined with immunohistochemistry and zymography. In that case, in situ zymography provides data that extend our understanding of the role of specific proteinases in various physiological and pathological conditions.

(J Histochem Cytochem 52:711–722, 2004)

Key Words: proteinase • gelatinase • in situ zymography • metabolic mapping

	Introduction

Top Summary Introduction Metabolic Mapping of Protease... Zymography In Situ Zymography of... In Situ Zymography with... In Situ Zymography with... Literature Cited

 
A PROTEASE can be defined as an enzyme that hydrolyzes peptide bonds. Proteases can be divided into endopeptidases or proteinases, which cleave internal peptide bonds in proteins, and exopeptidases, which cleave terminal peptide bonds. Exopeptidases can be further subdivided into aminopeptidases and carboxypeptidases, depending on which end of the protein amino acids are cleaved off. Proteases can be classified as aspartic proteases (e.g., cathepsins D and E, pepsin, renin), cysteine proteases (e.g., cathepsins B, L, S, K, Q, calpains, and caspases), metalloproteases (e.g., gelatinases A and B), serine proteases (e.g., plasminogen activators, plasmin, and chymase), and threonine proteases (e.g., proteasome), depending on the nature of the active site. Selective inhibitors can be used to distinguish among these classes of proteases. Protease activity is regulated in vivo by altering the rate of their synthesis and degradation, activation of (pre-)proforms, and binding with endogenous inhibitors.

Initially, proteases were considered as hydrolytic enzymes that were associated with protein catabolism, but it is now widely accepted that the highly specific hydrolysis of peptide bonds can regulate a wide range of biological processes (e.g., via processing of bioactive peptides) in all living organisms. This highly specific substrate cleavage is referred to as proteolytic processing, which regulates the activity and the compartmentalization of many proteins and therefore of many cellular processes (Barrett et al. 1998; Lopez-Otin and Overall 2002). Dysregulation of protease expression and in particular of their activity is involved in various pathological conditions, such as cardiovascular and neurodegenerative diseases, arthritic diseases, infection, and cancer. Therefore, proteases are attractive potential therapeutic targets.

Various techniques are used to determine the presence of proteases in tissues. Northern blotting analysis and RT-PCR are applied to quantify mRNAs in tissue extracts, whereas in situ hybridization (ISH) is used to localize mRNA in cell preparations or tissue sections. However, transcriptional activity does not necessarily reflect the amount and activity of the protein product of a certain gene. Western blots and immunohistochemistry (IHC) are used to determine the amount and localization of the protease protein but do not provide information about the activity of a protease because proteases are synthetized in an inactive proform or preproform that requires proteolytic processing for activation. Moreover, endogenous protease inhibitors can bind proteases and inhibit them. Biochemical techniques have been developed to detect protease activity in tissue extracts. However, homogenization of tissues for these assays does not allow localization of enzyme activity. In addition, extraction procedures can artifactually activate enzymes or cause interactions of active enzymes with their respective inhibitors when they are localized in different compartments in intact tissues. Therefore, techniques to localize specific proteolytic activity in cell preparations or tissue sections may provide crucial additional information on the exact role played by proteases in various physiological and pathological conditions.

	Metabolic Mapping of Protease Activity

Top Summary Introduction Metabolic Mapping of Protease... Zymography In Situ Zymography of... In Situ Zymography with... In Situ Zymography with... Literature Cited

 
Over 30 years ago, Robert E. Smith and colleagues developed synthetic substrates for specific proteinases with the leaving group 4-methoxy-2-naphthylamine (MNA; Smith et al. 1972; Smith and Van Frank 1975). The substrates consist of the MNA-leaving group attached to an amino acid sequence specific for the proteinase under study (Lojda 1984). The latter can be coupled after proteolytic removal of the amino acids either to a diazonium salt, such as Fast Blue BB, to give a colored final reaction product (Lojda 1984), to hexazotized pararosanilin or new fuchsin for electron microscopic purposes (Schroeder and Gossrau 1982), or to 5-nitrosalicylaldehyde, which results in a yellow fluorescent reaction product (Dolbeare and Smith 1977). Figure 1 shows the ultrastructural localization of cathepsin B activity in lysosomes of rat liver parenchymal cells, as demonstrated with Z-ala-arg-arg-MNA as substrate and hexazotized pararosanilin as coupling reagent. The procedure was performed as described by Schellens et al. (2003).

View larger version (153K): [in this window] [in a new window]   Figure 1 Electron micrograph of an unfixed, permeabilized, isolated liver parenchymal cell incubated for demonstration of cathepsin B activity with Z-ala-arg-arg-4-methoxy-2-naphthylamide as substrate and hexazotized p-rosanilin as coupling reagent. After incubation, cells were fixed in a mixture of glutaraldehyde and formaldehyde, postfixed in a solution of osmium tetroxide, and embedded in Epon. Final reaction product is localized exclusively in lysosomes. Bar = 0.5 µm.

It is becoming increasingly recognized that enzymes may behave differently in living cells and tissues than in frozen or fixed cells or tissue sections. Therefore, techniques are being developed for the detection of protease activities, such as those of dipeptidyl peptidase IV (DPPIV) and cathepsin B in living cells (Van Noorden et al. 1997,1998). A review on fluorogenic substrates available for metabolic mapping in living cells was recently published (Boonacker and Van Noorden 2001). Rhodamine-based fluorogenic dipeptide substrates were first synthesized by Leytus et al. (1983) for aminopeptidase, DPPIV, cathepsin B, cathepsin K, and cathepsin L. Recently, a new type of fluorogenic substrate for proteases has been synthetized based on the leaving group cresyl violet (Van Noorden et al. 1997,1998; Lee et al. 2003). The methods to localize protease activity in living cells using cresyl violet-based and rhodamine-based substrates have been critically evaluated by Boonacker et al. (2003).

Fluorogenic substrates for caspases are based on peptide sequences that are 18 amino acids long containing motifs that are specifically recognized by caspases and two identical fluorophores covalently attached near their termini. In such dimers, the fluorophore fluorescence is 90% quenched and fluorescence is generated when the substrate is cleaved (Komoriya et al. 2000; Kohler et al. 2002). The same type of substrate with quenched fluorogenic properties is also available for cathepsin D and MMP-2 (Bremer et al. 2001a,b). Thus far, these methods have been applied to living cells. Whether the localization of the final fluorescent reaction product is precisely enough to localize protease activity in tissue sections has yet to be established.

Proteolysis in tumor cells has been used by Weissleder et al. (1999) to develop an in vivo imaging system for tumors. An optimally quenched near-infrared fluorescence (NIRF) probe generates a strong NIRF signal after proteolytic activation. The probe is cleaved by lysosomal cysteine and serine proteases. This approach may also provide perspectives for localization of protease activities in tissue sections.

An entirely different approach to demonstrate activated caspases in living cells is the use of Caspa Tags, which are carboxyfluorescein-labeled fluoromethylketone inhibitors (Kohler et al. 2002). These cell-permeable inhibitors bind more or less specifically and irreversibly to the active site of caspases. Because the active site is available only in mature caspases, the Caspa Tags can exclusively stain cells containing the processed caspases of interest and the probes will not accumulate in normal (non-apoptotic) cells. This principle may have applications for the demonstration of other active proteases as well.

In conclusion, reliable techniques are available for the demonstration of activities of cysteine proteinases, serine proteinases, and aspartic proteinases using artificial substrates that contain small numbers of peptides, but demonstration of activities of MMPs with these small substrates had only limited success owing to the large numbers of peptide bonds that can be cleaved by MMPs and the overlap among different MMPs.

	Zymography

Top Summary Introduction Metabolic Mapping of Protease... Zymography In Situ Zymography of... In Situ Zymography with... In Situ Zymography with... Literature Cited

 
Zymography is a simple, sensitive, quantifiable, and functional approach for the analysis of proteolytic activity in cell and tissue extracts, which was introduced more that 20 years ago (Heussen and Dowdle 1980). It is widely used to study extracellular matrix (ECM)-degrading enzymes, in particular the MMPs. MMPs are zinc-dependent endopeptidases capable of degrading ECMs, including the basement membrane. The MMP family consists of at least 26 members and has been classified into subgroups on the basis of substrate preference and molecular structure. These are interstitial collagenases, gelatinases, stromelysins, and matrilysins, although all enzymes have overlapping substrate specificity. A recently discovered MMP family consists of membrane-type MMPs that are characterized by a transmembrane domain or a GPI-anchor (Visse and Nagase 2003).

The standard method for zymography is based on the use of SDS-polyacrylamide gels co-polymerized with a protein substrate, in particular gelatin, casein, or fibrin. Proteases that have the ability to renature after removal of SDS and to exert proteolytic activity on a co-polymerized substrate can be analyzed with this method. MMP-2 (gelatinase A, 72 kD) and MMP-9 (gelatinase B, 92 kD) can be detected on gelatin zymograms and MMP-7 on casein gels. Coomassie Blue staining of the gel reveals sites of proteolysis as white bands on a dark blue background. Figure 2 shows a zymogram of a homogenate of a tumor of colon cancer cells in mouse liver containing four bands responsible for gelatin breakdown. Based on the molecular weights, these bands reflect inactive and active MMP-2 and inactive and active MMP-9 (Ackema, unpublished results). Polyacrylamide gel co-polymerization with plasminogen and gelatin allows detection of the plasminogen activators urokinase-type plasminogen activator (uPA) and tissue-type plasminogen activator (tPA) as plasmin generated by uPA and/or tPA degrades gelatin (Figure 3 ; Leber and Balkwill 1997). Casein zymography has been used as an alternative assay for fibrinolytic enzymes because of the ability of plasmin to degrade casein. Kim et al. (1998) introduced fibrin zymography to detect fibrinolytic enzymes by incorporating fibrinogen and thrombin into SDS polyacrylamide gels. Although gelatin and casein are satisfactory substrates for plasmin, all fibrinolytic enzymes are not able to cleave these substrates as plasmin is. Apparently, fibrin is an in vivo substrate for plasmin and plasmin-like enzymes that can be demonstrated reliably with fibrin zymography.

View larger version (30K): [in this window] [in a new window]   Figure 2 Gelatin zymography of a homogenate of colon cancer metastases in mouse liver. ProMMP-9 (92 kD), proMMP-2 (72 kD), active MMP-9 (82 kD), and active MMP-2 (62 kD) are present.

View larger version (10K): [in this window] [in a new window]   Figure 3 Principle of detection of activity of urokinase-type plasminogen activator (uPA) and tissue-type plasminogen activator (tPA).

It can be concluded that zymography enables the detection of protease activity in cell or tissue homogenates using gelatin, casein, or fibrin as substrates. On the basis of molecular weight markers, the molecular weight of the proteolytic band can be determined, and by comparison with recombinant proteins and the use of specific protease inhibitors the type of protease can be established. However, information on the localization of the proteolytic activity in cells or tissues cannot be obtained on the basis of zymography.

	In Situ Zymography of Gelatinase Activity

Top Summary Introduction Metabolic Mapping of Protease... Zymography In Situ Zymography of... In Situ Zymography with... In Situ Zymography with... Literature Cited

 
During the past decade, in situ zymography has been applied to localize gelatinase activity in tissue sections (Galis et al. 1994). This method is based on the principle of gel substrate zymography. Galis et al. (1994)(1995) used gelatin that contains fluorescein or an autoradiographic emulsion as substrate layer on cryostat sections of human atherosclerotic plaques to assess gelatinolytic activity in situ. Autoradiographic emulsions were introduced because gelatin is the main component of the emulsion and gelatinolytic activity during incubation results in decreased amounts of silver in specific sites that can be visualized by photographic development. Microscopy reveals transparent spots on top of the areas with gelatinolytic activity against a black background (Galis et al. 1994). Fluorescein-coupled gelatin was introduced to try to improve the precision of localization of gelatinolytic activity because disappearance of fluorescence indicates areas with gelatinolytic activity (Galis et al. 1995). Because fluorescein is a fluorophore that does not have optimal fluorescent properties for microscopy, Oregon Green conjugates were introduced, which have similar spectral characteristics as fluorescein, but their fluorescence is more photostable and less pH-dependent than fluorescein (Pirila et al. 2001; Faia et al. 2002).

The principle introduced by Galis et al. (1995) has been modified in the procedure to demonstrate breakdown of gelatin differently. Instead of fluorescent gelatin, some authors used pure gelatin that was stained after incubation with Ponceau S (Loy et al. 2002), amido black (Ikeda et al. 2000; Furuya et al. 2001), or Biebrich Scarlet (Wada et al. 2003). Another approach based on zymography was used by Kurschat et al. (2002), who incorporated gelatin into polyacrylamide gels of 50 µm thickness, which were brought into contact with unfixed cryostat sections. After incubation, sections and gels were separated and gels were stained with Coomassie Blue. All the approaches have in common the fact that a decrease in staining intensity is a reflection of gelatinolytic activity. Details of the principles of photographic emulsion-based and fluorescently-labeled substrate-based in situ zymography were recently reviewed by Yan and Blomme (2003). These authors concluded that the photographic emulsion technique was more sensitive than the fluorescent gelatin principle.

The approach of gelatin in situ zymography has been applied to study involvement of gelatinolytic activity in many (patho)physiological processes in tissues such as arteries (Knox et al. 1997; Bruno et al. 1998; Faia et al. 2002), veins (Fernandez et al. 1998; George et al. 1998; Kranzhofer et al. 1999), heart (Tyagi et al. 1996; Robert et al. 1997), lung (Pardo et al. 1996; Leco et al. 2001), skin (Fisher et al. 1997; Krejci-Papa and Paus 1998), eye (Zhou et al. 1998; Hanyu 1999), equine hoof (Mungall et al. 1998; Mungall and Pollitt 1999,2001), joints (Freemont et al. 1999; Yamanaka et al. 2000), colon (Tarlton et al. 2000), muscle (Kieseier et al. 2001), nerve (Duchossoy et al. 2001; Siebert et al. 2001), ovary (Curry et al. 2001; Khandoker et al. 2001), gingiva (Pirila et al. 2001), adipocytes (Maquoi et al. 2002), and endometrium (Zhang and Salamonsen 2002; Zheng et al. 2002). All studies indicate that gelatinases have a role in remodeling and/or degradation of the ECM.

Based on the high-level expression and proenzyme activation of gelatinases in tumors, in situ zymography has been used to study the involvement of gelatinolytic activity in cancer progression. Gelatinolytic activity was demonstrated in a series of human malignancies such as those of ovary (Furuya et al. 2001; Lengyel et al. 2001), cervix (Minami et al. 2003), breast (Iwata et al. 2001), lung (Ikeda et al. 2000; Kaji et al. 2003), thyroid (Nakamura et al. 1999), esophagus (Koyama et al. 2000), oral cavity (Shimada et al. 2000), brain (Nakada et al. 1999), kidney (Kamiya et al. 2003), and liver (Kaneyoshi et al. 2001). In almost all cases, MMP-2 appeared to be responsible for gelatinolytic activity and the activity was presumed to be related to the invasive and metastatic properties of the cancers.

The approach that was used in these studies was reduction in staining intensity of the gels on top of the sections. This approach has two major disadvantages. First, sensitivity of reduction in staining intensity is less than that of formation of staining and, second, it is doubtful whether this principle can be used for quantitative purposes (Thomas et al. 1998; Mungall and Pollitt 2001). Therefore, other procedures were developed in which a colored or fluorescent product was formed at the site of gelatinolytic activity. Ratnikov et al. (2000) introduced biotinylated gelatin as a substrate to demonstrate gelatinolytic activity in solution. After cleavage of the substrate, the proteolytic fragments bearing the biotin moieties are captured by streptavidin coated on the plastic surface of a 96-well microtiter plate. Activity of horseradish peroxidase conjugated to streptavidin is measured. This biotinylated gelatin may also have perspectives for in situ localization when diaminobenzidine or aminoethylcarbazole is used to localize peroxidase activity.

The application of gelatin as substrate for in situ zymography has the advantage that, as far as we know, only MMP-2 and MMP-9 have a high affinity for this substrate. However, definite conclusions about the specific enzyme(s) responsible for gelatin breakdown can be drawn only when selective inhibitors are used and the in situ zymography is combined with gelatin zymography and IHC of MMP-2, MMP-9, and other potential gelatin-degrading enzymes. Gelatin zymography enables the assessment of molecular weights of the proteins that degrade gelatin. Moreover, differences in molecular weight of proenzymes and activated enzymes allow estimation of relative amounts of proenzymes and active enzymes in homogenates of tissues under study.

It can be concluded that in situ zymography with gelatin as substrate enables the localization of MMP activities, but thus far precise localization is not possible.

	In Situ Zymography with Quenched Fluorogenic DQ-gelatin

Top Summary Introduction Metabolic Mapping of Protease... Zymography In Situ Zymography of... In Situ Zymography with... In Situ Zymography with... Literature Cited

 
Precise localization of gelatinase activity in sections and cells became possible with the introduction of dye-quenched (DQ)-gelatin, which is gelatin that is heavily labeled with FITC molecules so that its fluorescence is quenched (Oh et al. 1999; Curry et al. 2001; Duchossoy et al. 2001; Goodall et al. 2001; Lindsey et al. 2001; Teesalu et al. 2001; Wang and Lakatta 2002; Zhang and Salamonsen 2002; Mook et al. 2003; Platt et al. 2003; Lee et al. 2004). After cleavage of DQ-gelatin by gelatinolytic activity, fluorescent peptides are produced that can be visualized against a weakly fluorescent background (EnzCheck; Molecular Probes, Eugene, OR). The substrate was developed for assaying protease activity in solutions, but the substrate has properties that enable localization of protease activity in cells or tissues under certain conditions. Oh et al. (1999) incubated unfixed cryostat sections of developing optic nerves and cultured live oligodendrocytes with an aqueous medium containing DQ-gelatin. After overnight incubation without any further fixation or washes, gelatinolytic activity was localized and photographed. This procedure enabled localization of MMP-2 and MMP-9 activity in developing optic nerves. It appeared that the activity had a similar distribution pattern as myelin basic protein. Activity was also found pericellularly at growing tips of oligodendrocytes. Formation of fluorescent peptides was prevented by addition of phenanthroline or TIMP-1 to the incubation media, which indicates that MMP activity was demonstrated. Parallel investigations on MMP-2 and MMP-9 of oligodendrocytes with zymography led to the conclusion that MMP-9 was the gelatinase involved in myelin formation by oligodendrocytes. The same procedure was recently applied by Lee et al. (2004), who localized gelatinolytic activity due to MMP-9 in pyramidal and granular neurons of the hippocampus after ischemia. An important role for MMP-9 in the pathogenesis of neuronal damage was proposed. Curry et al. (2001) added 1% agarose to DQ-gelatin in analogy with the principle introduced by Galis et al. (1995). After spreading this solution on glass slides and gelling at 4C, unfixed cryostat sections were mounted on the gelatin substrate, coverslipped, and incubated for 20 hr at 37C. Fluorescence was detected in rat ovaries during follicular growth, ovulation, and early luteal formation. Production of fluorescence was prevented by EDTA and ilomastat, a synthetic MMP inhibitor. Therefore, it was concluded that gelatinolytic activity by MMPs was demonstrated in these tissues. Teesalu et al. (2001) used DQ-gelatin, agar, and unfixed cryostat sections to localize gelatinolytic activity in inflammatory lesions caused by experimental autoimmune encephalomyelitis and demonstrated that MMP-9 was responsible for the in situ gelatin breakdown on the basis of parallel zymography experiments.

MMP-9 activity was detected in the vicinity of infiltrating neutrophils in canine myocardium subjected to ischemia and reperfusion with the use of DQ-gelatin applied to unfixed cryostat sections (Lindsey et al. 2001). Gelatinolytic activity was inhibited by both EDTA and neutralizing MMP-9 antibody. Moreover, gelatinolytic activity was not observed in non-ischemic myocardium. It was concluded that infiltrating neutrophils were the source of active MMP-9.

MMP-2 activity was localized on elastin fibers in blood vessel walls after incubation of cryostat sections of inferior mesenteric veins of patients with abdominal aortic aneurysms with DQ-gelatin (Goodall et al. 2001). Phenanthroline inhibited production of fluorescence and gelatin zymography demonstrated the presence of active MMP-2. The authors concluded that MMP-2 plays a primary role in aneurysm formation. However, it should be noted that autofluorescence of elastin fibers may interfere with detection of fluorescence due to gelatinolytic activity.

Duchossoy et al. (2001) combined in situ zymography using DQ-gelatin with immunodetection of laminin to study the role of MMPs in spinal cord injury. For this purpose, unfixed spinal cord cryostat sections were incubated overnight in medium containing DQ-gelatin and antibody against laminin. After a rapid wash, sections were incubated with secondary antibodies and studied with fluorescence microscopy. Gelatinolytic activity was co-localized with laminin surrounding blood vessels in injured spinal cord and was detected in lesion sites in and around infiltrating cells. Preincubation with blocking antibodies against MMP-2 and MMP-9 strongly reduced fluorescence intensity, suggesting the involvement of gelatinase activity. The authors concluded that gelatinases play a role in blood–spinal barrier disruption, leukocyte infiltration, disruption of the ECM, and clearance of debris after spinal cord injury. Because it is difficult to imagine that soluble fluorescent peptides produced by cleavage of DQ-gelatin can be detected after a wash of the sections and additional incubation with secondary antibodies, it must be concluded that extracellular localization of gelatinase activity must be the result of binding of fluorescent peptides to MMPs in the ECM.

Zhang and Salamonsen (2002) were not successful in combining in situ zymography using DQ-gelatin and immunostaining of MMPs on the same section of human endometrium. This may be due to the fact that cryostat sections were fixed in formalin and 2% gelatin was added to the DQ-gelatin-containing incubation medium. It has been established that fixation with formaldehyde and therefore no doubt with formalin, completely inhibits gelatinolytic activity (Mook et al. 2003). Moreover, the addition of 2% gelatin to 0.01% DQ-gelatin may reduce the efficacy of breakdown of DQ-gelatin. In situ zymography without simultaneous IHC detection of MMP-2 and MMP-9 resulted in findings on the basis of which it was concluded that MMPs were more active in menstrual endometrium compared with other stages of the cycle, which suggests that MMPs play a role in matrix degradation during menstruation. Wang and Lakatta (2002) demonstrated gelatinolytic activity to be increased in the wall of rat aortas in relation with aging using DQ-gelatin. However, detailed descriptions of the method they applied were lacking. It was concluded that activity mainly resulted from MMP-2 because activity was almost completely inhibited by a blocking antibody against MMP-2. The role of MMP-2 and MMP-9 in rat sciatic nerves after crush and during regeneration was established with in situ zymography with DQ-gelatin and gel zymography (Platt et al. 2003). The fluorescence due to gelatinase activity at the lesion site was prevented by addition of phenanthroline.

The first application to cancer of in situ zymography with DQ-gelatin was performed by Mook et al. (2003). The procedure was based on the incubation of unfixed cryostat sections of rat liver containing colon cancer metastases using a low-gelling temperature (LGT) agar- and DQ-gelatin-containing incubation medium. The time of incubation was only 60 min, the method could be combined with IHC on the same section, and the method was extensively tested for its specificity. Gelatinolytic activity due to MMP-2 was detected in stroma of colon cancer metastases (Figure 4) .

View larger version (123K): [in this window] [in a new window]   Figures 4 and 5 Figure 4 In situ zymography of gelatinolytic activity with DQ-gelatin as substrate in colon cancer metastasis in rat liver. Fluorescence due to gelatinolytic activity (green) was found in the extracellular matrix of tumors. Nuclei are shown in red. Bar = 35 µm. Figure 5 In situ zymography of urokinase-type plasminogen activator activity with Bodipy-casein as substrate and added plasminogen in colon cancer metastasis in mouse liver. Fluorescence due to caseinolytic activity (red) was found in intratumoral stroma of tumors. Nuclei are shown in green. Bar = 35 µm.

	In Situ Zymography with Other Quenched Fluorogenic Substrates

Top Summary Introduction Metabolic Mapping of Protease... Zymography In Situ Zymography of... In Situ Zymography with... In Situ Zymography with... Literature Cited

 
Most studies performed thus far with in situ zymography using quenched fluorogenic substrates dealt with gelatinolytic activity. However, other quenched fluorogenic substrates are also available. These are DQ-collagen type I, DQ-collagen type IV, DQ-elastin, DQ-bovine serum albumin (BSA), DQ-ovalbumin, and DQ-casein (Jones et al. 1997). These substrates were initially developed to demonstrate activity of proteinases in solution. However, the substrates can in principle be used also to detect proteinase activity in unfixed cryostat sections or cell preparations when LGT-agar or another gelling compound is added to the incubation medium. It must be emphasized that development of other natural substrates of MMPs with quenched fluorescence, such as laminins and fibronectins, should be encouraged.

DQ-collagen type I was applied to fixed cryostat sections of endometrial biopsy specimens in the presence of gelatin (Zhang and Salamonsen 2002). Collagenase activity was observed in small foci within the tissue in all phases of the menstrual cycle, but collagenase activity was most abundant premenstrually and during the menstrual phase. Collagenase activity was localized extracellularly and was abolished when sections were pretreated with phenanthroline. It was concluded that MMP-1 was responsible for the breakdown of collagen type I because the protein showed a similar localization pattern. MMPs appear to play a critical role in matrix degradation during menstruation.

DQ-collagen type IV has been mainly applied to cells cultured on matrices containing the substrate (Horino et al. 2001; Sameni et al. 2001; Elner 2002; Premzl et al. 2003). Invasion of fibrosarcoma cells in gelatin matrix was accompanied by collagenolytic activity due to MMP activity (Horino et al. 2001). Sameni et al. (2000)(2001) investigated the site of proteolysis in a three-dimensional gelatin matrix embedded with DQ-collagen type IV and human cancer cells cultured on top of it. Cells at all levels in the matrix accumulated fluorescent degradation products of DQ-collagen IV intracellularly in vesicles. Based on findings using inhibitors, it was concluded that lysosomal proteinases, such as cathepsin B, are responsible for intracellular degradation of collagen type IV in human breast cancer cells, glioma cells, and colon cancer cells, and are involved in cancer cell invasion.

A similar approach was used by Premzl et al. (2003), who localized the breakdown of DQ-collagen IV by ras-transformed breast cancer cells during invasion in matrigel. Intracellular and extracellular cleavage of collagen type IV was detected that was largely due to intracellular and extracellular cathepsin B activities. Yan and Blomme (2003) demonstrated breakdown of DQ-collagen type IV in cryostat sections of rat tibia. Fluorescence was observed in the distal portion of the hypertrophic zone of growth plates of the tibia. MMP-9 was held responsible for collagenolytic activity because EDTA prevented the production of fluorescence, and protein and mRNA of MMP-9 were similarly localized as the fluorescence due to collagen type IV breakdown.

In situ zymography of uPA was introduced by Sappino et al. (1991) using plasminogen and casein as substrate. Plasminogen was converted by uPA to plasmin, which degraded casein. de Vries et al. (1995) demonstrated with this approach uPA activity in sprouting capillaries in melanomas. The production of fluorescent peptides from DQ-casein was recently used for the precise localization of uPA activity in unfixed cryostat sections of mouse liver with colon cancer metastases (Ackema, unpublished results). Figure 5 shows the localization of fluorescent breakdown products of Bodipy-casein in colon cancer metastases of mouse liver. DQ-BSA has also been used instead of DQ-casein as substrate for the localization of uPA activity in matrices containing fibrosarcoma cells (Horino et al. 2001) and retinal pigment cells (Elner 2002). The specificity of extracellular proteolysis of BSA by uPA was assessed by inhibition with PAI-1. BSA can be cleaved by many proteinases and specificity tests are therefore very important. Koblinski et al. (2000) showed that intracellular cathepsin B is responsible for the intracellular accummulation of degraded DQ-BSA in transfected fibroblasts grown on a gelatin matrix containing DQ-BSA.

Summarizing, dye-quenched fluorogenic natural substrates other than gelatin have mainly been used in gel matrices containing cultured cells and have rarely been applied to cryostat sections. The use of these substrates has potential for the localization of activity of proteinases, but it should be emphasized that proper controls must be performed to establish the proteinases involved, such as the use of inhibitors and combination with detection methods such as IHC and zymography.

In conclusion, precise localization of proteinase activity using natural substrates containing quenched fluorescence is a valuable tool to study its role in (patho)physiological processes. The value of the method may even increase when fluorescence production can be measured locally. Fluorescence should then be measured locally during incubation, and measurements should fulfill a series of criteria as formulated by Stoward (1980), as has been established for many other enzyme histochemical procedures (Van Noorden and Frederiks 1992). Moreover, in situ zymography localization should be combined with IHC, preferably on the same sections or at least on serial sections. Finally, zymography of cell or tissue homogenates should also be performed to assess the nature of the protein and, as a consequence, the type of proteinase that cleaves the substrate.

Protocol 1
This is the method of choice to detect gelatinolytic activity with in situ zymography and DQ-gelatin in cells or tissues.

1. Dissolve 1 g LGT agarose in 100 ml PBS, pH 7.45, under continuous stirring and heating in a water bath (80C) until a clear solution is obtained.
   
2. Store the clear agarose-containing solution at 4C in air-tight vials.
   
3. Heat the agarose-containing solution to 60C to obtain a clear solution before incubation.
   
4. Cool the desired volume of the solution to 37C before incubation.
   
5. DQ-gelatin (Molecular Probes) is dissolved in a concentration of 1 mg/ml in distilled water.
   
6. The DQ-gelatin solution is diluted 1:10 in the agarose-containing solution.
   
7. Use unfixed cells or unfixed cryostat sections of the tissue to be investigated (8–10 µm thick).
   
8. The DQ-gelatin agarose mixture (40 µl) is put on top of the dried cells or sections and covered with a coverslip of 24 x 40 mm.
   
9. The agar is gelled at 4C.
   
10. Incubation is performed for 1–24 hr at RT dependent on the enzyme activity.
    
11. Fluorescence of FITC is detected with excitation at 460–500 nm and emission at 512–542 nm.
    
12. Control incubations should be carried out on cells or serial cryostat sections by adding 20 mM EDTA or a selective MMP inhibitor to the incubation medium.
    
13. Cells or sections should be preincubated for 1 hr at RT with the different inhibitors dissolved in PBS.
    
14. The presence of autofluorescence in cells or sections should be tested by incubating in the agarose-containing medium that lacks DQ-gelatin.
    
15. Nuclei can be counterstained by adding DAPI (1 µg/ml) or propidium iodide (0.5 µg/ml) to the incubation medium.
    
16. Analyze the cells of sections: compare the fluorescence of FITC formed after incubation in the presence of DQ-gelatin with the fluorescence produced after incubation in the absence of DQ-gelatin or in the presence of DQ-gelatin and MMP inhibitors.
    

Protocol 2
This is the procedure of choice to detect gelatinolytic activity with in situ zymography in cells or tissues in combination with IHC.

1. Cells or cryostat sections are air-dried for 1 hr at RT.
   
2. Cells or cryostat sections are fixed in acetone for 10 min at RT. Crosslinking fixatives should be avoided, because they affect enzyme activity.
   
3. The IHC procedure for the desired antigen is performed according to standard procedures using a fluorescently labeled secondary antibody with spectral properties other than FITC.
   
4. The procedure as described in protocol 1 is performed to detect gelatinolytic activity.
   
5. Analyze the cells or sections: compare the localization of the fluorescence of FITC with that of the other fluorophore.
   

	Acknowledgments

 
We are grateful to Prof Dr C.J.F. Van Noorden for most valuable comments on the manuscript. We wish to thank Ms H. Vreeling and Ms E. Ackema for providing their micrographs, Mr J. Peeterse for preparation of the micrographs, and Ms T.M.S. Pierik for careful preparation of the manuscript.

	Footnotes

 
Received for publication January 7, 2004; accepted February 27, 2004

	Literature Cited

Top Summary Introduction Metabolic Mapping of Protease... Zymography In Situ Zymography of... In Situ Zymography with... In Situ Zymography with... Literature Cited

 

Barrett AJ, Rawlings ND, Woessner JF (1998) Handbook of Proteolytic Enzymes. 1st ed. London, Academic Press

Boonacker E, Elferink S, Bardai A, Fleischer B, Van Noorden CJ (2003) Fluorogenic substrate [Ala-Pro]2-cresyl violet but not Ala-Pro-rhodamine 110 is cleaved specifically by DPPIV activity: a study in living Jurkat cells and CD26/DPPIV-transfected Jurkat cells. J Histochem Cytochem 51:959–968[Abstract/Free Full Text]

Boonacker E, Van Noorden CJ (2001) Enzyme cytochemical techniques for metabolic mapping in living cells, with special reference to proteolysis. J Histochem Cytochem 49:1473–1486[Abstract/Free Full Text]

Bremer C, Bredow S, Mahmood U, Weissleder R, Tung CH (2001a) Optical imaging of matrix metalloproteinase-2 activity in tumors: feasibility study in a mouse model. Radiology 221:523–529[Abstract/Free Full Text]

Bremer C, Tung CH, Weissleder R (2001b) In vivo molecular target assessment of matrix metalloproteinase inhibition. Nature Med 7:743–748[CrossRef][Medline]

Bruno G, Todor R, Lewis I, Chyatte D (1998) Vascular extracellular matrix remodeling in cerebral aneurysms. J Neurosurg 89:431–440[Medline]

Catterall JB, Cawston TE (2003) Assays of matrix metalloproteinases (MMPs) and MMP inhibitors: bioassays and immunoassays applicable to cell culture medium, serum, and synovial fluid. Methods Mol Biol 225:353–364[Medline]

Curry TE Jr, Song L, Wheeler SE (2001) Cellular localization of gelatinases and tissue inhibitors of metalloproteinases during follicular growth, ovulation, and early luteal formation in the rat. Biol Reprod 65:855–865[Abstract/Free Full Text]

de Vries TJ, Kitson JL, Silvers WK, Mintz B (1995) Expression of plasminogen activators and plasminogen activator inhibitors in cutaneous melanomas of transgenic melanoma-susceptible mice. Cancer Res 55:4681–4687[Abstract/Free Full Text]

Dolbeare FA, Smith RE (1977) Flow cytometric measurement of peptidases with use of 5-nitrosalicylaldehyde and 4-methoxy-beta-naphthylamine derivatives. Clin Chem 23:1485–1491[Abstract/Free Full Text]

Duchossoy Y, Arnaud S, Feldblum S (2001) Matrix metalloproteinases: potential therapeutic target in spinal cord injury. Clin Chem Lab Med 39:362–367[CrossRef][Medline]

Elner SG (2002) Human retinal pigment epithelial lysis of extracellular matrix: functional urokinase plasminogen activator receptor, collagenase, and elastase. Trans Am Ophthalmol Soc 100:273–299[Medline]

Faia KL, Davis WP, Marone AJ, Foxall TL (2002) Matrix metalloproteinases and tissue inhibitors of metalloproteinases in hamster aortic atherosclerosis: correlation with in-situ zymography. Atherosclerosis 160:325–337[CrossRef][Medline]

Fernandez HA, Kallenbach K, Seghezzi G, Mehrara B, Apazidis A, Baumann FG, Grossi EA, et al. (1998) Modulation of matrix metalloproteinase activity in human saphenous vein grafts using adenovirus-mediated gene transfer. Surgery 124:129–136[Medline]

Fisher GJ, Wang ZQ, Datta SC, Varani J, Kang S, Voorhees JJ (1997) Pathophysiology of premature skin aging induced by ultraviolet light. N Engl J Med 337:1419–1428[Abstract/Free Full Text]

Freemont AJ, Byers RJ, Taiwo YO, Hoyland JA (1999) In situ zymographic localisation of type II collagen degrading activity in osteoarthritic human articular cartilage. Ann Rheum Dis 58:357–365[Abstract/Free Full Text]

Furuya M, Ishikura H, Nemori R, Shibata M, Fujimoto S, Yoshiki T (2001) Clarification of the active gelatinolytic sites in human ovarian neoplasms using in situ zymography. Hum Pathol 32:163–168[CrossRef][Medline]

Galis ZS, Sukhova GK, Lark MW, Libby P (1994) Increased expression of matrix metalloproteinases and matrix degrading activity in vulnerable regions of human atherosclerotic plaques. J Clin Invest 94:2493–2503

Galis ZS, Sukhova GK, Libby P (1995) Microscopic localization of active proteases by in situ zymography: detection of matrix metalloproteinase activity in vascular tissue. FASEB J 9:974–980[Abstract]

George SJ, Baker AH, Angelini GD, Newby AC (1998) Gene transfer of tissue inhibitor of metalloproteinase-2 inhibits metalloproteinase activity and neointima formation in human saphenous veins. Gene Ther 5:1552–1560[CrossRef][Medline]

Goodall S, Crowther M, Hemingway DM, Bell PR, Thompson MM (2001) Ubiquitous elevation of matrix metalloproteinase-2 expression in the vasculature of patients with abdominal aneurysms. Circulation 104:304–309[Abstract/Free Full Text]

Hanyu T (1999) The effects of single mitomycin C application on the expression of matrix metalloproteinase in the sclera and aqueous of albino rabbits. Nippon Ganka Gakkai Zasshi 103:186–192[Medline]

Heussen C, Dowdle EB (1980) Electrophoretic analysis of plasminogen activators in polyacrylamide gels containing sodium dodecyl sulfate and copolymerized substrates. Anal Biochem 102:196–202[CrossRef][Medline]

Horino K, Kindezelskii AL, Elner VM, Hughes BA, Petty HR (2001) Tumor cell invasion of model 3-dimensional matrices: demonstration of migratory pathways, collagen disruption, and intercellular cooperation. FASEB J 15:932–939[Abstract/Free Full Text]

Ikeda M, Maekawa R, Tanaka H, Matsumoto M, Takeda Y, Tamura Y, Nemori R, et al. (2000) Inhibition of gelatinolytic activity in tumor tissues by synthetic matrix metalloproteinase inhibitor: application of film in situ zymography. Clin Cancer Res 6:3290–3296[Abstract/Free Full Text]

Iwata H, Yamamoto M, Nemori R, Mizutani M, Iwase T, Miura S, Obata Y, et al. (2001) Localization of gelatinolytic activity can be detected in breast cancer tissues by film in situ zymography. Breast Cancer 8:111–115[Medline]

Jones LJ, Upson RH, Haugland RP, Panchuk-Voloshina N, Zhou M (1997) Quenched BODIPY dye-labeled casein substrates for the assay of protease activity by direct fluorescence measurement. Anal Biochem 251:144–152[CrossRef][Medline]

Kaji M, Moriyama S, Sasaki H, Saitoh Y, Kiriyama M, Fukai I, Yamakawa Y, et al. (2003) Gelatinolytic activity of matrix metalloproteinase in lung cancer studied using film in situ zymography stamp method. Lung Cancer 39:125–130[CrossRef][Medline]

Kamiya N, Kishimoto T, Suzuki H, Sekita N, Nagai Y, Oosumi N, Kito H, et al. (2003) Increased in situ gelatinolytic activity in renal cell tumor tissues correlates with tumor size, grade and vessel invasion. Int J Cancer 106:480–485[CrossRef][Medline]

Kaneyoshi T, Nakatsukasa H, Higashi T, Fujiwara K, Naito I, Nouso K, Kariyama K, et al. (2001) Actual invasive potential of human hepatocellular carcinoma revealed by in situ gelatin zymography. Clin Cancer Res 7:4027–4032[Abstract/Free Full Text]

Khandoker MA, Imai K, Takahashi T, Hashizume K (2001) Role of gelatinase on follicular atresia in the bovine ovary. Biol Reprod 65:726–732[Abstract/Free Full Text]

Kieseier BC, Schneider C, Clements JM, Gearing AJ, Gold R, Toyka KV, Hartung HP (2001) Expression of specific matrix metalloproteinases in inflammatory myopathies. Brain 124:341–351[Abstract/Free Full Text]

Kim SH, Choi NS, Lee WY (1998) Fibrin zymography: a direct analysis of fibrinolytic enzymes on gels. Anal Biochem 263:115–116[CrossRef][Medline]

Knox JB, Sukhova GK, Whittemore AD, Libby P (1997) Evidence for altered balance between matrix metalloproteinases and their inhibitors in human aortic diseases. Circulation 95:205–212[Abstract/Free Full Text]

Koblinski JE, Ahram M, Sloane BF (2000) Unraveling the role of proteases in cancer. Clin Chim Acta 291:113–135[CrossRef][Medline]

Kohler C, Orrenius S, Zhivotovsky B (2002) Evaluation of caspase activity in apoptotic cells. J Immunol Methods 265:97–110[CrossRef][Medline]

Komoriya A, Packard BZ, Brown MJ, Wu ML, Henkart PA (2000) Assessment of caspase activities in intact apoptotic thymocytes using cell-permeable fluorogenic caspase substrates. J Exp Med 191:1819–1828[Abstract/Free Full Text]

Koyama H, Iwata H, Kuwabara Y, Iwase H, Kobayashi S, Fujii Y (2000) Gelatinolytic activity of matrix metalloproteinase-2 and -9 in oesophageal carcinoma; a study using in situ zymography. Eur J Cancer 36:2164–2170

Kranzhofer A, Baker AH, George SJ, Newby AC (1999) Expression of tissue inhibitor of metalloproteinase-1, -2, and -3 during neointima formation in organ cultures of human saphenous vein. Arterioscler Thromb Vasc Biol 19:255–265[Abstract/Free Full Text]

Krejci-Papa NC, Paus R (1998) A novel in-situ-zymography technique localizes gelatinolytic activity in human skin to mast cells. Exp Dermatol 7:321–326[CrossRef][Medline]

Kurschat P, Wickenhauser C, Groth W, Krieg T, Mauch C (2002) Identification of activated matrix metalloproteinase-2 (MMP-2) as the main gelatinolytic enzyme in malignant melanoma by in situ zymography. J Pathol 197:179–187[CrossRef][Medline]

Leber TM, Balkwill FR (1997) Zymography: a single-step staining method for quantitation of proteolytic activity on substrate gels. Anal Biochem 249:24–28[CrossRef][Medline]

Leco KJ, Waterhouse P, Sanchez OH, Gowing KL, Poole AR, Wakeham A, Mak TW, et al. (2001) Spontaneous air space enlargement in the lungs of mice lacking tissue inhibitor of metalloproteinases-3 (TIMP-3). J Clin Invest 108:817–829[CrossRef][Medline]

Lee BW, Johnson GL, Hed SA, Darzynkiewicz Z, Talhouk JW, Mehrotra S (2003) DEVDase detection in intact apoptotic cells using the cell permeant fluorogenic substrate, (z-DEVD)2-cresyl violet. BioTechniques 35:1080–1085[Medline]

Lee SR, Tsuji K, Lee SR, Lo EH (2004) Role of matrix metalloproteinases in delayed neuronal damage after transient global cerebral ischemia. J Neurosci 24:671–678[Abstract/Free Full Text]

Lengyel E, Schmalfeldt B, Konik E, Spathe K, Harting K, Fenn A, Berger U, et al. (2001) Expression of latent matrix metalloproteinase 9 (MMP-9) predicts survival in advanced ovarian cancer. Gynecol Oncol 82:291–298[CrossRef][Medline]

Leytus SP, Melhado LL, Mangel WF (1983) Rhodamine-based compounds as fluorogenic substrates for serine proteinases. Biochem J 209:299–307[Medline]

Lindsey M, Wedin K, Brown MD, Keller C, Evans AJ, Smolen J, Burns AR, et al. (2001) Matrix-dependent mechanism of neutrophil-mediated release and activation of matrix metalloproteinase 9 in myocardial ischemia/reperfusion. Circulation 103:2181–2187[Abstract/Free Full Text]

Lojda Z (1984) Histochemistry of proteases. Acta Histochem 30:9–28

Lojda Z (1996) The use of substrates with 7-amino-3-trifluoromethylcoumarine (AFC) leaving group in the localization of protease activities in situ. Acta Histochem Armed Forces Inst. of Pathology 98:215–228

Lopez-Otin C, Overall CM (2002) Protease degradomics: a new challenge for proteomics. Nature Rev Mol Cell Biol 3:509–519[CrossRef][Medline]

Loy M, Burggraf D, Martens KH, Liebetrau M, Wunderlich N, Bultemeier G, Nemori R, et al. (2002) A gelatin in situ-overlay technique localizes brain matrix metalloproteinase activity in experimental focal cerebral ischemia. J Neurosci Methods 116:125–133[CrossRef][Medline]

Maquoi E, Munaut C, Colige A, Collen D, Lijnen HR (2002) Modulation of adipose tissue expression of murine matrix metalloproteinases and their tissue inhibitors with obesity. Diabetes 51:1093–1101[Abstract/Free Full Text]

Minami R, Tsunoda H, Iijima T, Yoshikawa H, Nemori R, Noguchi M (2003) Early acquisition of gelatinolytic activity in carcinogenesis of the uterine cervix. Mod Pathol 16:1164–1170[CrossRef][Medline]

Mook OR, Van Overbeek C, Ackema EG, Van Maldegem F, Frederiks WM (2003) In situ localization of gelatinolytic activity in the extracellular matrix of metastases of colon cancer in rat liver using quenched fluorogenic DQ-gelatin. J Histochem Cytochem 51:821–829[Abstract/Free Full Text]

Mungall BA, Pollitt CC, Collins R (1998) Localisation of gelatinase activity in epidermal hoof lamellae by in situ zymography. Histochem Cell Biol 110:535–540[CrossRef][Medline]

Mungall BA, Pollitt CC (1999) Zymographic analysis of equine laminitis. Histochem Cell Biol 112:467–472[CrossRef][Medline]

Mungall BA, Pollitt CC (2001) In situ zymography: topographical considerations. J Biochem Biophys Methods 47:169–176[CrossRef][Medline]

Nakada M, Nakamura H, Ikeda E, Fujimoto N, Yamashita J, Sato H, Seiki M, et al. (1999) Expression and tissue localization of membrane-type 1, 2, and 3 matrix metalloproteinases in human astrocytic tumors. Am J Pathol 154:417–428[Abstract/Free Full Text]

Nakamura H, Ueno H, Yamashita K, Shimada T, Yamamoto E, Noguchi M, Fujimoto N, et al. (1999) Enhanced production and activation of progelatinase A mediated by membrane-type 1 matrix metalloproteinase in human papillary thyroid carcinomas. Cancer Res 59:467–473[Abstract/Free Full Text]

Oh LY, Larsen PH, Krekoski CA, Edwards DR, Donovan F, Werb Z, Yong VW (1999) Matrix metalloproteinase-9/gelatinase B is required for process outgrowth by oligodendrocytes. J Neurosci 19:8464–8475[Abstract/Free Full Text]

Pardo A, Selman M, Ridge K, Barrios R, Sznajder JI (1996) Increased expression of gelatinases and collagenase in rat lungs exposed to 100% oxygen. Am J Respir Crit Care Med 154:1067–1075[Abstract]

Pirila E, Maisi P, Salo T, Koivunen E, Sorsa T (2001) In vivo localization of gelatinases (MMP-2 and -9) by in situ zymography with a selective gelatinase inhibitor. Biochem Biophys Res Commun 287:766–774[CrossRef][Medline]

Platt CI, Krekoski CA, Ward RV, Edwards DR, Gavrilovic J (2003) Extracellular matrix and matrix metalloproteinases in sciatic nerve. J Neurosci Res 74:417–429[CrossRef][Medline]

Premzl A, Zavasnik-Bergant V, Turk V, Kos J (2003) Intracellular and extracellular cathepsin B facilitate invasion of MCF-10A neoT cells through reconstituted extracellular matrix in vitro. Exp Cell Res 283:206–214[CrossRef][Medline]

Ratnikov B, Deryugina E, Leng J, Marchenko G, Dembrow D, Strongin A (2000) Determination of matrix metalloproteinase activity using biotinylated gelatin. Anal Biochem 286:149–155[CrossRef][Medline]

Ratnikov BI, Deryugina EI, Strongin AY (2002) Gelatin zymography and substrate cleavage assays of matrix metalloproteinase-2 in breast carcinoma cells overexpressing membrane type-1 matrix metalloproteinase. Lab Invest 82:1583–1590[Medline]

Robert V, Besse S, Sabri A, Silvestre JS, Assayag P, Nguyen VT, Swynghedauw B, et al. (1997) Differential regulation of matrix metalloproteinases associated with aging and hypertension in the rat heart. Lab Invest 76:729–738[Medline]

Sameni M, Dosescu J, Sloane BF (2001) Imaging proteolysis by living human glioma cells. Biol Chem 382:785–788[CrossRef][Medline]

Sameni M, Moin K, Sloane BF (2000) Imaging proteolysis by living human breast cancer cells. Neoplasia 2:496–504[CrossRef][Medline]

Sappino AP, Belin D, Huarte J, Hirschel-Scholz S, Saurat JH, Vassalli JD (1991) Differential protease expression by cutaneous squamous and basal cell carcinomas. J Clin Invest 88:1073–1079

Schellens JP, Vreeling-Sindelarova H, Frederiks WM (2003) Electron microscopical enzyme histochemistry on unfixed tissues and cells. Bridging the gap between LM and EM enzyme histochemistry. Acta Histochem 105:1–19[CrossRef][Medline]

Schroeder J, Gossrau R (1982) Electron microscopic localization of proteases by the direct azo dye staining method. Acta Histochem 25:147–152

Shimada T, Nakamura H, Yamashita K, Kawata R, Murakami Y, Fujimoto N, Sato H, et al. (2000) Enhanced production and activation of progelatinase A mediated by membrane-type 1 matrix metalloproteinase in human oral squamous cell carcinomas: implications for lymph node metastasis. Clin Exp Metastasis 18:179–188[CrossRef][Medline]

Siebert H, Dippel N, Mader M, Weber F, Bruck W (2001) Matrix metalloproteinase expression and inhibition after sciatic nerve axotomy. J Neuropathol Exp Neurol 60:85–93[Medline]

Smith RE, Smithwick EL, Allen CH (1972) A new assay for cathepsin B1 using CBZ-Ala-Arg-Arg-4-Me0-ß-NA. J Histochem Cytochem 20:843

Smith RE, Van Frank RM (1975) The use of amino acid derivatives of 4-methoxy-ß-naphthylamine for the assay and subcellular localization of tissue proteinases. In Dingle JT, Dean RJ, eds. Lysosomes in Biology and Pathology. Amsterdam, North-Holland, 193

Stoward PJ (1980) Criteria for the validation of quantitative histochemical enzyme techniques. In Everid D, O'Connor M, eds. Trends in Enzyme Histochemistry and Cytochemistry. Amsterdam, Excerpta Medica, 11–31

Tarlton JF, Whiting CV, Tunmore D, Bregenholt S, Reimann J, Claesson MH, Bland PW (2000) The role of up-regulated serine proteases and matrix metalloproteinases in the pathogenesis of a murine model of colitis. Am J Pathol 157:1927–1935[Abstract/Free Full Text]

Teesalu T, Hinkkanen AE, Vaheri A (2001) Coordinated induction of extracellular proteolysis systems during experimental autoimmune encephalomyelitis in mice. Am J Pathol 159:2227–2237[Abstract/Free Full Text]

Thomas M, Barker G, Furness PN (1998) A semi-quantitative approach to in situ zymography using tissue sections. J Pathol 186:4A

Tyagi SC, Kumar SG, Haas SJ, Reddy HK, Voelker DJ, Hayden MR, Demmy TL, et al. (1996) Post-transcriptional regulation of extracellular matrix metalloproteinase in human heart end-stage failure secondary to ischemic cardiomyopathy. J Mol Cell Cardiol 28:1415–1428[CrossRef][Medline]

Van Noorden CJ, Boonacker E, Bissell ER, Meijer AJ, van Marle J, Smith RE (1997) Ala-Pro-cresyl violet, a synthetic fluorogenic substrate for the analysis of kinetic parameters of dipeptidyl peptidase IV (CD26) in individual living rat hepatocytes. Anal Biochem 252:71–77[CrossRef][Medline]

Van Noorden CJ, Jonges TG, Van Marle J, Bissell ER, Griffini P, Jans M, Snel J, et al. (1998) Heterogeneous suppression of experimentally induced colon cancer metastasis in rat liver lobes by inhibition of extracellular cathepsin B. Clin Exp Metastasis 16:159–167[CrossRef][Medline]

Van Noorden CJ, Vogels IM, Everts V, Beertsen W (1987) Localization of cathepsin B activity in fibroblasts and chondrocytes by continuous monitoring of the formation of a final fluorescent reaction product using 5-nitrosalicylaldehyde. Histochem J 19:483–487[CrossRef][Medline]

Van Noorden CJ, Vogels IM, Smith RE (1989) Localization and cytophotometric analysis of cathepsin B activity in unfixed and undecalcified cryostat sections of whole rat knee joints. J Histochem Cytochem 37:617–624[Abstract]

Van Noorden CJF, Frederiks WM (1992) Enzyme Histochemistry. A Laboratory Manual of Current Methods. Oxford, Oxford University Press

Visse R, Nagase H (2003) Matrix metalloproteinases and tissue inhibitors of metalloproteinases: structure, function, and biochemistry. Circ Res 92:827–839[Abstract/Free Full Text]

Wada N, Otani Y, Kubota T, Kimata M, Minagawa A, Yoshimizu N, Kameyama K, et al. (2003) Reduced angiogenesis in peritoneal dissemination of gastric cancer through gelatinase inhibition. Clin Exp Metastasis 20:431–435[CrossRef][Medline]

Wang M, Lakatta EG (2002) Altered regulation of matrix metalloproteinase-2 in aortic remodeling during aging. Hypertension 39:865–873[Abstract/Free Full Text]

Weissleder R, Tung CH, Mahmood U, Bogdanov A Jr (1999) In vivo imaging of tumors with protease-activated near-infrared fluorescent probes. Nature Biotechnol 17:375–378[CrossRef][Medline]

Yamanaka H, Makino K, Takizawa M, Nakamura H, Fujimoto N, Moriya H, Nemori R, et al. (2000) Expression and tissue localization of membrane-types 1, 2, and 3 matrix metalloproteinases in rheumatoid synovium. Lab Invest 80:677–687[Medline]

Yan SJ, Blomme EA (2003) In situ zymography: a molecular pathology technique to localize endogenous protease activity in tissue sections. Vet Pathol 40:227–236[CrossRef][Medline]

Yi CF, Gosiewska A, Burtis D, Geesin J (2001) Incorporation of fluorescent enzyme substrates in agarose gel for in situ zymography. Anal Biochem 291:27–33[CrossRef][Medline]

Zhang J, Salamonsen LA (2002) In vivo evidence for active matrix metalloproteinases in human endometrium supports their role in tissue breakdown at menstruation. J Clin Endocrinol Metab 87:2346–2351[Abstract/Free Full Text]

Zheng K, Nagai Y, Kishimoto T, Yamazawa K, Tate S, Nemori R, Hirai Y, et al. (2002) A quantitative evaluation of active gelatinolytic sites in uterine endometrioid adenocarcinoma using film in situ zymography: association of stronger gelatinolysis with myometrial invasion. Jpn J Cancer Res 93:516–522[CrossRef][Medline]

Zhou L, Sawaguchi S, Twining SS, Sugar J, Feder RS, Yue BY (1998) Expression of degradative enzymes and protease inhibitors in corneas with keratoconus. Invest Ophthalmol Vis Sci 39:1117–1124[Abstract/Free Full Text]

Zucker S, Lysik RM, Gurfinkel M, Zarrabi MH, Stetler-Stevenson W, Liotta LA, Birkedal-Hansen H, et al. (1992) Immunoassay of type IV collagenase/gelatinase (MMP-2) in human plasma. J Immunol Methods 148:189–198[CrossRef][Medline]

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