Abstract
BackgroundVirus-binding activity is one of the important functions of fibronectin (FN). It has been reported that a high concentration of FN in blood improves the transmission frequency of hepatitis viruses. Therefore, to investigate a protease that hydrolyzes FN rapidly is useful to decrease the FN concentration in blood and HBV infection. So far, however, no specific protease digesting FN in serum has been reported.MethodsWe employed a purified earthworm protease to digest serum proteins. The rapidly cleaved protein (FN) was identified by MALDI-TOF MS and western blotting. The cleavage sites were determined by N-terminus amino acid residues sequencing. The protease was orally administrated to rats to investigate whether serum FN in vivo became decreased. The serum FN was determined by western blotting and ELISA. In cytological studies, the protease was added to the medium in the culture of HepG2.2.15 cells and then HBsAg and HBeAg were determined by ELISA.ResultsThe protease purified from earthworm Eisenia fetida was found to function as a fibronectinase (FNase). The cleavage sites on FN by the FNase were at R and K, exhibiting a trypsin alkaline serine-like function. The earthworm fibronectinase (EFNase) cleaved FN at four sites, R259, R1005, K1557 and R2039, among which the digested fragments at R259, K1557 and R2039 were related to the virus-binding activity as reported. The serum FN was significantly decreased when the earthworm fibronectinase was orally administrated to rats. The ELISA results showed that the secretion of HBeAg from HepG2.2.15 cells was significantly inhibited in the presence of the FNase.ConclusionThe earthworm fibronectinase (EFNase) cleaves FN much faster than the other proteins in serum, showing a potential to inhibit HBV infection through its suppressing the level of HBeAg. This suggests that EFNase is probably used as one of the candidates for the therapeutic agents to treat hepatitis virus infection.
Highlights
Virus-binding activity is one of the important functions of fibronectin (FN)
earthworm fibronectinase (EFNase) and lamivudine were added to the media 3 days after seeding
EFNase was incubated with human serum (25 μl) at different time intervals during the degradation and aliquots were taken for SDS-PAGE
Summary
It has been reported that a high concentration of FN in blood improves the transmission frequency of hepatitis viruses. To investigate a protease that hydrolyzes FN rapidly is useful to decrease the FN concentration in blood and HBV infection. Each subunit is a mosaic of a series of repeating modules: 12 Type I, 2 Type II, 15 to 17 (depending on splicing) Type III modules, and a variable (V) sequence that is not homologous to other parts of FN. Plasma FN that is synthesized in hepatocytes contains neither EDA nor EDB whereas cellular FN (synthesized locally in tissues) contains variable amounts of either or both EDA and EDB. Plasma FN is an abundant soluble constituent in plasma with a concentration about 300 μg/ml [1]; and cellular FN is an extracellular matrix that provides the architectural scaffolding in tissues [3]
Sign-in/Register to view highlights & summary 
Published Version (
Free)
Talk to us
Join us for a 30 min session where you can share your feedback and ask us any queries you have
Schedule a call