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Computational design of Matrix Metalloprotenaise-9 (MMP-9) resistant to auto-cleavage
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AbstractMatrix metalloproteinase-9 (MMP-9) is an endopeptidase that remodels the extracellular matrix and has been implicated as a major driver in cancer metastasis. Hence, there is a high demand for MMP-9 inhibitors for therapeutic purposes. For such drug design efforts, large amounts of MMP-9 are required. Yet, the catalytic domain of MMP-9 (MMP-9Cat) is an intrinsically unstable enzyme that tends to auto-cleave within minutes, making it difficult to use in drug design experiments and other biophysical studies. We set our goal to design MMP-9Catvariant that is active but stable to autocleavage. For this purpose, we first identified potential autocleavage sites on MMP-9Catusing mass spectroscopy and then eliminated the autocleavage site by predicting mutations that minimize autocleavage potential without reducing enzyme stability. Four computationally designed MMP-9Catvariants were experimentally constructed and evaluated for auto-cleavage and enzyme activity. Our best variant, Des2, with 2 mutations, was as active as the wild-type enzyme but did not exhibit auto-cleavage after seven days of incubation at 37°C. This MMP-9Catvariant, with an identical to MMP- 9CatWT active site, is an ideal candidate for drug design experiments targeting MMP-9 and enzyme crystallization experiments. The developed strategy for MMP-9CATstabilization could be applied to redesign of other proteases to improve their stability for various biotechnological applications.
Cold Spring Harbor Laboratory
Title: Computational design of Matrix Metalloprotenaise-9 (MMP-9) resistant to auto-cleavage
Description:
AbstractMatrix metalloproteinase-9 (MMP-9) is an endopeptidase that remodels the extracellular matrix and has been implicated as a major driver in cancer metastasis.
Hence, there is a high demand for MMP-9 inhibitors for therapeutic purposes.
For such drug design efforts, large amounts of MMP-9 are required.
Yet, the catalytic domain of MMP-9 (MMP-9Cat) is an intrinsically unstable enzyme that tends to auto-cleave within minutes, making it difficult to use in drug design experiments and other biophysical studies.
We set our goal to design MMP-9Catvariant that is active but stable to autocleavage.
For this purpose, we first identified potential autocleavage sites on MMP-9Catusing mass spectroscopy and then eliminated the autocleavage site by predicting mutations that minimize autocleavage potential without reducing enzyme stability.
Four computationally designed MMP-9Catvariants were experimentally constructed and evaluated for auto-cleavage and enzyme activity.
Our best variant, Des2, with 2 mutations, was as active as the wild-type enzyme but did not exhibit auto-cleavage after seven days of incubation at 37°C.
This MMP-9Catvariant, with an identical to MMP- 9CatWT active site, is an ideal candidate for drug design experiments targeting MMP-9 and enzyme crystallization experiments.
The developed strategy for MMP-9CATstabilization could be applied to redesign of other proteases to improve their stability for various biotechnological applications.
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