Tissue plasminogen activator ( t-PA ) produced by IMR-90 ( human embryonic fibroblast
) cells cultured in the serum-free medium ( DMEM ) containing 1% proteos^e peptone
and 1.6 - 3.6mM CaCl2 was purified by the procedure consisted of ultrafiltration, immunoadsorpt ion chromatography,
HPLC and lysine-Sepharose chromatography. The yield of t-PA from the culture broth
was approximately 47%. The purified t-PA migrated as a single band on SDS-polyacrylamide
gels. The molecular weight of the t-PA was estimated to be 66,000 by SDS-polyacrylamide
gel electrophoresis and 69,000 by gel filtration method. Purified t-PA had a specific
activity of 36 × 104 IU/mg protein by fiblin plate method or 54 - 56 X 104 IU/mg protein by clot lysis method using t-PA obtained from WHO as a standard. The
amino acid composition of fibroblast t-PA was very similar to those of melanoma t-PA
and uterine t-PA. Isoelectric point of fibroblast t-PA ranged from 5-7 to 8.2. The
t-PA had twice as much affinity for fiblin as did high molecular weight urokinase
( UK ). Both t-PA and UK had optimum temperature at 41°C and optimum pH between 8.0
- 9.0. The polyclonal and monoclonal antibodies raised against t-PA quenched t-PA
activity but had no effect on UK activity. The inhibitors of serine proteases, difluorophos-phate
and gabexate mesilate, strongly inhibited the activities of fibroblast t-PA and UK.
The nucleotide sequence analysis of the t-PA cDNA isolated from the cDNA library prepared
from IMR-90 mRNA revealed the nucleotide changes at two positions in the coding region
as compared to that of melanoma t-PA cDNA. Neither of the changes replaced the coded
amino acid. The N-terminal amino acid of fibroblast t-PA was determined to be valine,
indicatig the structural similarity of fibroblast t-PA to uterine t-PA.
