Development of subunit selective proteasome substrates forSchistosoma species

Author:

Jiang ZhenzeORCID,Silva Elany B.ORCID,Liu Chenxi,Fajtová PavlaORCID,Liu Lawrence J.,El-Sakkary NellyORCID,Skinner Danielle E.,Syed Ali,Wang Steven C,Caffrey Conor R.ORCID,O’Donoghue Anthony J.ORCID

Abstract

AbstractSchistosomiasis, or bilharzia, is a neglected tropical disease caused bySchistosomaspp. blood flukes that infects over 200 million people worldwide. Just one partially effective drug is available, and new drugs and drug targets would be welcome. The 20S proteasome is a validated drug target for many parasitic infections, including those caused byPlasmodiumandLeishmania. We previously showed that anticancer proteasome inhibitors that act through theSchistosoma mansoni20S proteasome (Sm20S) kill the parasitein vitro. To advance these initial findings, we employed Multiplex Substrate Profiling by Mass Spectrometry (MSP-MS) to define the substrate cleavage specificities of the three catalytic β subunits of purified Sm20S. The profiles in turn were used to design and synthesize subunit-specific optimized substrates that performed two to eight fold better than the equivalent substrates used to measure the activity of the constitutive human proteasome (c20S). These specific substrates also eliminated the need to purify Sm20S from parasite extracts - a single step enrichment was sufficient to accurately measure substrate hydrolysis and its inhibition with proteasome inhibitors. Finally, we show that the substrate and inhibition profiles for the 20S proteasome from the three medically important schistosome species are similar, suggesting that data arising from an inhibitor development campaign that focuses on Sm20S can be extrapolated to the other two targets with consequent time and cost savings.

Publisher

Cold Spring Harbor Laboratory

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