Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Pivot Concepts:
Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Target Concepts:
Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Query: EC:3.4.21.4 (
trypsin
)
42,187
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Collagenase released from embryonic and adult human skin explants has been studied with special reference to the latency of the enzyme. 1) Embryonic human skin explants showed a much higher capacity for collagenase production than did adult skin, on the basis of unit weight of tissue. 2) Culture medium from embryonic skin explants contained latent collagenase at almost twice the concentration of the active form. No appreciable amount of latent enzyme was observed in the adult skin system. 3) The molecular weights of active and latent collagenases were about 40,000 and 50,000, respectively. 4) The latent collagenase was found to be activated by simple passage through a Sephadex G-50 column after adding
NaI
to a final concentration of 3 M. The degree of activation produced by this treatment was as high as that by limited proteolysis with
trypsin
. It was concluded that no activating enzyme system was involved in the activation of latent collagenase during
NaI
treatment, and that the latent enzyme was composed of an enzyme-inhibitor complex. 5) The physiological significance of latent enzyme in the regulation of collagenase activity in vivo is discussed.
...
PMID:A latent collagenase from embryonic human skin explants. 19 62
The [3H] phlorizin-binding component of brush border vesicles was enriched in situ by negative purification. Several procedures, known to effect selective solubilization of membrane components, were used separately or in combination to remove proteins unrelated to the binding. Deoxycholate ruptured the vesicles and released 67% of their protein, thereby increasing the specific [3H] phlorizin-binding activity of the pellet three-to fourfold. Extracting the deoxycholate-pellets with either
NaI
or alkaline solutions released up to 38% of the deoxycholate-insoluble protein without significantly affecting phlorizin binding. The polypeptide composition of the membranes at the different stages was analyzed by NaDodSO4-polyacrylamide gel electrophoresis. A number of polypeptides present in the original vesicles could be ruled out as essential components of the [3H] phlorizin binding entity. Intact and deoxycholate-treated vesicles were subjected to proteolytic attack. Papain liberated sucrase and isomaltase from intact vesicles, but affected neither other Coomassie-stained bands nor phlorizin binding. Neither the protein composition nor the binding properties of sealed vesicles were influenced by
trypsin
or chymotrypsin. However, all the proteolytic enzymes tested on deoxycholate-treated membranes substantially reduced [3H] phlorizin binding and produced concomitantly the disappearance of several bands from the electrophoretic profile. Pretreatment of vesicles with papain, followed by deoxycholate extraction and incubation in alkaline media, increased the specific binding activity of the membranes up to ninefold by removing close to 90% of the protein. A limited number of polypeptides are suggested as possible candidates for the glycoside-binding site of intestinal brush borders.
...
PMID:Partial purification of the sugar carrier of intestinal brush border membranes. Enrichment of the phlorizin-binding component by selective extractions. 52 29
The Mg-adenosinetriphosphatase (ATPase) in the thyroidal
NaI
-treated microsome fraction was activated by treatment with basic polyamino acids or
trypsin
, but not with acidic polyamino acids and basic proteins such as lysozyme and ribonuclease. The enzyme kinetics showed that the activation of
trypsin
or poly-L-lysine was due to an increase in the maximal velocity of the hydrolyzing reaction without a change in the affinity of the enzyme for its substrate. A break at about 25 degrees C was observed in the Arrhenius plots of Mg-ATPase in the
trypsin
- or poly-L-lysine treated preparations, but there was no break in the control preparation. These results suggest that the activating effect of
trypsin
or poly-L-lysine on Mg-ATPase activity in the thyroidal
NaI
-treated microsome fraction is related to the lipid environment surrounding the enzyme molecule in the thyroid cell membrane.
...
PMID:Characterization of thyroidal membrane-bound Mg-adenosinetriphosphatase activated by trypsin or poly-L-lysine. 153 27
An antigen-specific method has been developed for direct detection and quantitation of HBsAg-ICs. The method involves (1) precipitation of HBsAg-ICs with 3.5% PEG; (2) dissociation of the PEG precipitated ICs by treatment with NaSCN,
NaI
, KBr, low or high pH buffers,
trypsin
or papain; and (3) detection and titration of HBsAg and/or anti-HBs liberated from ICs. Treatment with 2 M and 3 M NaSCN, papain or
trypsin
liberates HBsAg, while following treatment with 3 M and
NaI
free anti-HBs is detectable. Trypsin digestion (2 mg/ml, 30 min at 37 degrees C) proved to be most effective for disrupting HBsAg-ICs formed at equivalence as well as in excess of antigen or antibody. After
trypsin
digestion of the sample RPHA, RIA and ELISA may be used as a third step. Th
...
PMID:Detection and quantitation of hepatitis-B surface antigen immune complexes (HBsAg-ICs) by an antigen-specific method. I. Detection and quantitation of in vitro prepared HBsAg-ICs. 615 46
Latent and active forms of collagenase were detected in culture media of the normal rabbit colon. During culture, the collagenase appeared to be produced by surviving and growing mucosas on the degenerated or necrotic colon wall. Type III collagen was most readily degraded by the collagenase, followed by type I and II collagens. The collagenase did not attack type IV or V collagens. The latent collagenase was activated by
trypsin
and chaotropic agents such as 3 M NaSCN or
NaI
, and autoactivated gradually during storage. Activated latent collagenase showed the properties of metalloproteinase as in the active collagenase. The apparent molecular weights, determined by calibrated Sephadex G-75, were 39,000 and 31,000 for the latent and active enzymes, respectively. After 12 h of tissue culture, the latent collagenase appeared in the culture media 10-20 h earlier than the active collagenase. The collagenase in the culture media of the early period was mainly the latent form, while the media of the late period contained a large amount of the active form.
...
PMID:Collagenase from the culture medium of rabbit colon wall with special reference to the latent type and substrate specificity. 630 59
