Abstract
Differences evident in the sequence alignment of human cathepsin-L with shrimp cathepsin-L and silicatein-α suggest the indirect involvement of the heavy to light chain loop (E286 to E289) in the function of these enzymes. Deletion of the loop and adjacent residues S290 to N293, decreased specific protease activity by 81% and 63%, respectively; complete substitution for the corresponding silicatein-α loop decreased activity by 35%. In all cases the Km was largely unchanged. The conformational stability of human procathepsin-L was not altered by deletion of E286 to E289 but increased on deletion of S290 to N293. Therefore, shortening the loop does not change substrate affinity but does influence activity, in part via conformational change.
Keywords: Cathepsin-L, Silicatein-α, cysteine protease, protein engineering
Related Books
In Vitro Propagation and Secondary Metabolite Production from Medicinal Plants: Current Trends (Part 2)
Micropropagation of Medicinal Plants
Software and Programming Tools in Pharmaceutical Research
Biotechnology and Drug Development for Targeting Human Diseases
In Vitro Propagation and Secondary Metabolite Production from Medicinal Plants: Current Trends (Part 1)
Molecular and Physiological Insights into Plant Stress Tolerance and Applications in Agriculture- Part 2
Micropropagation of Medicinal Plants
Genome Editing in Bacteria (Part 1)
Data Science for Agricultural Innovation and Productivity
Animal Models In Experimental Medicine
17