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:3.4.23.5 (
cathepsin D
)
4,130
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Cathepsin D, an acidic protease normally acting in lysosomes, is overproduced both in vitro and in vivo in most breast cancer cells. The mechanism of gene regulation by estrogens and the biological and clinical significance of this overexpression in metastasis are reviewed. In MCF7 cells,
cathepsin D
is specifically and directly induced by estrogens and also induced by growth factors (EGF, IGF-I and
bFGF
), but this induction is dependent upon de novo protein synthesis. The mechanism of estrogen induction involves EREs located upstream from the gene. Our laboratory cloned the promoter region (-4kb) of
cathepsin D
of MCF7 cells and found EREs located in the proximal 5' region of the gene. In MDA-MB231 and BT20 cells,
cathepsin D
is overexpressed but not regulated by estrogens. Total
cathepsin D
concentration were assayed by IRMA in breast cancer cytosol routinely prepared for receptor assays. Several retrospective clinical studies indicate a significant correlation between high
cathepsin D
concentrations in the cytosol of primary breast cancer and further development of clinical metastasis. High
cathepsin D
concentration in the primary tumor may be either a consequence, or more likely a cause, of metastasis. Transfection experiments using cDNA-
cathepsin D
in rat tumoral cells facilitates their metastatic potential in nude mice (Garcia et al., Oncogene, 1990, 5, 1809-1814). The mechanism of
cathepsin D
action in facilitating metastasis is unknown and may involve proteolytic activity in an acidic compartment, and/or interaction with the Man 6P/IGFII receptor.
...
PMID:[Mechanism of the overexpression of the cathepsin D gene in breast cancer and consequences in the metastatic process]. 182 91
Mitogenic activity toward MCF-7 cells of two immunoreactive (high-molecular-weight form
bFGF
, HMW-
bFGF
; and 16-K
bFGF
, having the same molecular weight as recombinant
bFGF
) purified from pooled sera of breast cancer patients by heparin-affinity chromatography and gel filtration was investigated. The mitogenic activity of 16-K
bFGF
toward the cells was equal to that of recombinant
bFGF
, whereas the mitogenic effect of HMW-
bFGF
was weak. Most of the mitogenic activity of these two bFGFs was neutralized by anti-
bFGF
antibody. Also, the mitogenic activity of both HMW-
bFGF
and 16-K
bFGF
was markedly enhanced by aspartyl protease (
cathepsin D
), which is secreted in excess by breast cancer cells and is responsible for the enzymatic degradation of the extracellular matrix (ECM). By an enzyme immunoassay, we detected
cathepsin D
-mediated release of recombinant
bFGF
previously bound to the ECM of MCF-7 cells into the conditioned medium, and also observed
cathepsin D
-mediated proteolysis of HMW-
bFGF
to release free 16-K
bFGF
. These results suggest that 16-K
bFGF
is the
bFGF
molecule itself in the blood and that HMW-
bFGF
is a circulating form of
bFGF
in blood whose mitogenic activity is regulated by
cathepsin D
.
...
PMID:Mitogenic activity toward human breast cancer cell line MCF-7 of two bFGFs purified from sera of breast cancer patients: co-operative role of cathepsin D. 906 99
