Development of a novel, high-affinity ssDNA trypsin inhibitor

Malicki, Stanislaw; Ksiazek, Miroslaw; Majewski, Pawel; Pecak, Aleksandra; Mydel, Piotr; Grudnik, Przemyslaw; Dubin, Grzegorz

doi:10.6084/m9.figshare.7687139.v1

Development of a novel, high-affinity ssDNA trypsin inhibitor

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posted on 2019-02-07, 06:17 authored by Stanislaw Malicki, Miroslaw Ksiazek, Pawel Majewski, Aleksandra Pecak, Piotr Mydel, Przemyslaw Grudnik, Grzegorz Dubin

Inhibitors of serine proteases are not only extremely useful in the basic research but are also applied extensively in clinical settings. Using Systematic Evolution of Ligands by Exponential Enrichment (SELEX) approach we developed a family of novel, single-stranded DNA aptamers capable of specific trypsin inhibition. Our most potent candidate (T24) and its short version (T59) were thoroughly characterised in terms of efficacy. T24 and T59 efficiently inhibited bovine trypsin with K_i of 176 nM and 475 nM, respectively. Interestingly, in contrast to the majority of known trypsin inhibitors, the selected aptamers have superior specificity and did not interact with porcine trypsin or any human proteases tested. These included plasmin and thrombin characterised by trypsin-like substrate specificity. Our results demonstrate that SELEX may be successfully employed in the development of potent and specific DNA based protease inhibitors.

Funding

This work was supported by the National Science Centre, Poland, under Grants UMO-2013/08/W/NZ1/00696 and UMO-2011/01/D/NZ1/01169 (both to GD); the National Science Centre, Poland, under Grant UMO-2018/02/X/NZ1/02015 (to SM); the National Science Centre, Poland, under Grant UMO-2016/23/B/NZ5/011469 OPUS (to PM); Polish Ministry of Science and Higher Education—1306/MOB/IV/2015/0 (Mobility Plus to MK) and Uniwersytet Jagielloński w Krakowie.

Development of a novel, high-affinity ssDNA trypsin inhibitor

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