Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Pivot Concepts:
Gene/Protein
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Target Concepts:
Gene/Protein
Disease
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Drug
Enzyme
Compound
Query: EC:3.4.21.4 (
trypsin
)
42,187
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Recent evidence suggests that nonadrenergic airway relaxation may be controlled by vasoactive intestinal peptide (VIP). The magnitude and duration of smooth muscle relaxation in response to VIP may be influenced by rates of peptide degradation after release from efferent peptidergic neurons. To explore the potential role of mast cell mediators in modulating neural control of airway tone, we studied the effect of the mast cell proteases
tryptase
and chymase on airway smooth muscle relaxation induced by VIP in ferret airway. Tracheal rings precontracted by serotonin (10(-6) M) in a muscle bath were relaxed by VIP (10(-7) M). We found that protease-rich supernatant obtained by degranulation of dog mastocytoma cells reversed VIP-induced relaxation, as did highly purified
tryptase
and chymase incubated with the tracheal rings. Either enzyme completely reversed the effect of VIP, but
tryptase
was more potent than chymase, paralleling previous test tube observations on the relative rates of VIP cleavage by the two enzymes. Inhibitors of
mast cell tryptase
and chymase preincubated with the supernatant or with the purified proteases prevented reversal of VIP-induced relaxation. Mast cell proteases did not reverse the tracheal relaxation caused by the nonpeptide adrenergic agonist isoproterenol. These findings show that mast cell proteases
tryptase
and chymase counteract the smooth muscle relaxant effects of VIP in ferret trachea and suggest a potential role for the mast cell proteases in the modulation of nonadrenergic neural control of airway tone by VIP.
...
PMID:Mast cell tryptase and chymase reverse airway smooth muscle relaxation induced by vasoactive intestinal peptide in the ferret. 249 55
Mast cell tryptase is a secretory granule associated serine protease with
trypsin
-like specificity released extracellularly during mast cell degranulation. To determine the full primary structure of the catalytic domain and precursor forms of
tryptase
and to gain insight into its mode of activation, we cloned cDNAs coding for the complete amino acid sequence of dog
mast cell tryptase
and a second, possibly related, serine protease. Using RNA from dog mastocytoma cells, we constructed a cDNA library in lambda gt 10. Screening of the library with an oligonucleotide probe based on the N-terminal sequence of
tryptase
purified from the same cell source allowed us to isolate and sequence overlapping clones coding for dog
mast cell tryptase
. The
tryptase
sequence includes the essential residues of the catalytic triad and an aspartic acid at the base of the putative substrate binding pocket that confers P1 Arg and Lys specificity on tryptic serine proteases. The apparent N-terminal signal/activation peptide terminates in a glycine. A glycine in this position has not been observed previously in serine proteases and suggests a novel mode of activation. Additional screening of the library with a trypsinogen cDNA led to the isolation and sequencing of a full-length clone apparently coding for the complete sequence of a second tryptic serine protease (DMP) which is only 53.4% identical with the dog
tryptase
sequence but which contains an apparent signal/activation peptide also terminating in a glycine. Thus, the proteases encoded by these cloned cDNAs may share a common mode of activation from N-terminally extended precursors.
...
PMID:Molecular cloning of dog mast cell tryptase and a related protease: structural evidence of a unique mode of serine protease activation. 250 77
Crevicular fluid was collected from gingivitis and periodontitis patients on filter paper strips and then eluted into buffer. The eluates hydrolyzed ZAlaArgArgAFC at alkaline pH and the effector response at pH 8.5 indicated serine proteinase activity. The results, particularly the substantial increase in activity produced by heparin, were suggestive of
mast cell tryptase
. They were also consistent with the properties of the
tryptase
-like enzyme identified in extracts of inflamed human gingiva (Cox and Eley, Arch Oral Biol, in press). Partial inhibition of crevicular fluid eluate activity by soybean trypsin inhibitor suggested the additional presence of a second
trypsin
-like enzyme which might be of host or bacterial origin.
...
PMID:Tryptase-like activity in crevicular fluid from gingivitis and periodontitis patients. 252 68
The effect of human skin
mast cell tryptase
on human plasma proenzymes (prothrombin, coagulation factor XII, complement C1s, protein C and plasminogen) was investigated. Tryptase had no effect on these proenzymes, when incubated with them at 37 degrees C for up to 90 min, as judged by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and by the ability to hydrolyze specific peptide p-nitroanilide substrates. After prolonged treatment with
tryptase
, proenzymes could be fully activated with their specific activators. The results indicate that
tryptase
neither activates these plasma proenzymes nor inactivates the corresponding active enzymes. As a positive control, the
tryptase
preparation was also incubated with human fibrinogen and rat thymus histones. Prolonged treatment with
tryptase
increased the thrombin-induced clotting time of fibrinogen. Tryptase also efficiently hydrolyzed histone H1 from rat thymus. Histones H3/H2B and H2A were hydrolyzed less efficiently than H1, and no hydrolysis of histone H4 by
tryptase
was detected under the experimental conditions.
...
PMID:Effect of human mast cell tryptase on human plasma proenzymes. 253 Jan 78
Mast cells have been implicated in the pathogenesis of the matrix degradation observed in the cartilaginous and osseous structures of the rheumatoid joint. We previously reported that human
mast cell tryptase
, a 134-kD granule-associated neutral protease, is present in rheumatoid synovium and can activate collagenase in crude culture medium in vitro. the present study attempts to depict the precise mechanism of this activation. To express full activation of latent collagenase, matrix metalloproteinase 3 (MMP-3) or stromelysin, can be activated by
tryptase
in a time and dose-dependent manner. Tryptase was not capable of generating active collagenase in the crude media from cultured rheumatoid synoviocytes depleted of proMMP-3 by immunoadsorption. In addition, the function of the tissue inhibitor of metalloproteinases (TIMP) was not altered by
tryptase
, and SDS-PAGE analysis revealed no degradation of TIMP by
tryptase
. The
tryptase
dependent activation of synoviocyte procollagenase thereby appears to be entirely dependent upon its ability to activate proMMP-3.
...
PMID:Synovial procollagenase activation by human mast cell tryptase dependence upon matrix metalloproteinase 3 activation. 255 80
Supernatants obtained by degranulation of dog mastocytoma cells greatly increased the sensitivity and the magnitude of the contractile response of isolated dog bronchial smooth muscle to histamine. The enhanced contractile response was reversed completely by H1-receptor antagonists and was prevented by an inhibitor of
tryptase
(a major protease released with histamine from secretory granules of mast cells). The potentiation of histamine-induced contractions was reproduced by active
tryptase
in pure form. The contractions due to the combination of histamine and purified
tryptase
were abolished by the Ca2+ channel blockers nifedipine and verapamil. The bronchoconstricting effects of KCl and serotonin, which, like histamine, contract airway smooth muscle by a mechanism predominantly involving membrane potential-dependent Ca2+ transport, were also potentiated by
tryptase
. However, the contractile effects of acetylcholine, which contracts dog airway smooth muscle by a mechanism independent of Ca2+ channels, were unaffected by
tryptase
. These findings show a striking promotion of agonist-induced bronchial smooth muscle contraction by
mast cell tryptase
, via direct or indirect effects on Ca2+ channels, and the findings therefore suggest a novel potential mechanism of hyperresponsiveness in dog bronchi.
...
PMID:Mast cell tryptase causes airway smooth muscle hyperresponsiveness in dogs. 264 18
We tested four synthetic substances for their histochemical value to demonstrate the catalytic activities of chymase or
tryptase
in mast cells in sections of human gut. Both Suc-Ala-Ala-Phe-4 methoxy-2-naphthylamide (MNA) and N-acetyl-L-methionine-alpha-naphthyl ester (alpha-N-O-Met) reacted with chymase but not
tryptase
in mast cells. Conversely, D-Val-Leu-Arg-MNA and Z-Ala-Ala-Lys-MNA were hydrolyzed by
mast cell tryptase
but not chymase. These results were confirmed by use of two inhibitors of chymotrypsin-like activity, chymostatin and Z-Gly-Leu-Phe-chloromethyl ketone (CK) and two inhibitors of
trypsin
-like activity, Tos-Lys-CK and D-Val-Leu-Arg-CK. Excellent staining reactions were obtained on cryostat sections of unfixed or aldehyde-fixed tissues and on paraffin sections of Carnoy-fixed tissues. For chymase, however, Suc-Ala-Ala-Phe-MNA is preferred on cryostat sections because it is more specific. On paraffin sections alpha-N-O-Met is preferred because other cells are not then stained. For
tryptase
, Z-Ala-Ala-Lys-MNA was more selective and more specific and is the preferred general purpose substrate on cryostat sections of aldehyde-fixed tissues and for paraffin sections. D-Val-Leu-Arg-MNA is the preferred substrate for cryostat sections of unfixed tissue. Only a limited number of mast cells showed a reaction for chymase, and these occurred mainly in the submucosa. All mast cells, however, gave a reaction for
tryptase
, and we recommend the use of either substrate for this enzyme for routine detection of mast cells in human tissues. Double staining for the two main mast cell proteases is most conveniently undertaken on paraffin sections of Carnoy-fixed tissues using MNA substrates for
tryptase
and alpha-N-O-Met for chymase.
...
PMID:Enzyme histochemical discrimination between tryptase and chymase in mast cells of human gut. 264 38
The amino acid sequence of human
mast cell tryptase
was determined from corresponding cDNA cloned from a lambda ZAP library made with mRNA derived from a human mast cell preparation. Tryptase is the major neutral protease present in human mast cells and serves as a specific marker of mast cells by immunohistologic techniques and as a specific indicator of mast cell activation when detected in biologic fluids. Based on nucleic acid sequence, human
tryptase
consists of a 244-amino acid catalytic portion of 27,423 D with two putative N-linked carbohydrate binding sites and a 30-amino acid leader sequence of 3,048 D. A His74, Asp120, Ser223 catalytic triad and four cystine groups were identified by analogy to other serine proteases. Regions of amino acid sequence that are highly conserved in serine proteases, in general, were conserved in
tryptase
. The catalytic portion of human
tryptase
had an 84% amino acid sequence similarity with that of dog
tryptase
; their leader sequences had a 67% similarity. Asp217 in the substrate binding pocket of human
tryptase
is consistent with a specificity for Arg and Lys residues at the site of cleavage (P1), whereas Glu245 is consistent with the known preference of human
tryptase
for substrates with Arg or Lys also at P3, analogous residues also being present in dog
tryptase
. Asp244, which is substituted for the Gly found in dog
tryptase
and in most serine proteases, is present in the putative substrate binding pocket and may confer additional substrate specificity on human
tryptase
for basic residues. Further studies now can be designed to elucidate these structure-function relationships.
...
PMID:Cloning and characterization of complementary DNA for human tryptase. 267 49
The localization of
mast cell tryptase
in involved and noninvolved skin sections from 12 psoriatic patients was investigated using both enzyme- and immunohistochemical staining techniques. Each involved skin section contained an increased number of
tryptase
-positive mast cells in the superficial dermis as compared with corresponding noninvolved skin sections. The substrate-hydrolyzing and inhibition properties for
tryptase
activity in involved and non-involved psoriatic skin sections were identical with each other as well as with those previously described in normal human skin or mastocytoma skin sections. In four patients, epidermal enzyme activity was observed, but only in the involved skin. None of the uninvolved sections showed
tryptase
activity in the epidermis. This activity was not inhibited by alpha 1-antitrypsin, and after removing the enzyme-histochemical stain with Tween 20, positive results obtained with
tryptase
-specific antibody were found in the same locations. In addition,
tryptase
-positive cells were detected in close contact to lesional epidermis, but without epidermal staining in four patients. In the epidermis, the positive staining was granular, and active
tryptase
was detected as far as the stratum corneum. This study is the first description of the presence of active
mast cell tryptase
in psoriatic epidermis, where this enzyme may have a role in increased cell division.
...
PMID:Enzyme- and immunohistochemical localization of mast cell tryptase in psoriatic skin. 268 61
Pig synovial and human skin fibroblast procollagenases were treated with highly purified
tryptase
, the major proteinase of human mast cells, to determine whether this
trypsin
-like proteinase could activate the latent form of collagenase and so be involved in connective tissue breakdown. No significant activation of either human or pig procollagenase was found, but the highest concentration of
tryptase
partially destroyed procollagenase. Tryptase did not degrade type I collagen or proteoglycan. These data indicate that human
mast cell tryptase
does not contribute to connective tissue breakdown via procollagenase activation or via proteoglycan degradation.
...
PMID:Human lung mast cell tryptase fails to activate procollagenase or degrade proteoglycan. 299 69
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