FRET-Protease-Coupled Peptidyl-Prolyl cis-trans Isomerase Assay

Caporale, Andrea; Mascanzoni, Fabiola; Farina, Biancamaria; Sturlese, Mattia; Sorbo, Gianluigi Di; Fattorusso, Roberto; Ruvo, Menotti; Doti, Nunzianna

doi:10.1177/1087057116650402

Cited by 7 publications

(2 citation statements)

References 24 publications

(56 reference statements)

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“…We have tested this hypothesis using a CypA peptide substrate 25 and performing binding experiments between wild type and R55A mutant protein and the substrate in the presence and absence of the AIF(370-394) and CsA. Data showed that, in line with the large difference in affinity (57 nM for the substrate and 6 μM for the AIF peptide), AIF(370-394), used at a 10-fold excess, is unable to prevent the binding of both CypA and CypA R55A to the substrate, but recognition is abolished in the presence of the strong inhibitor CsA (Supplementary Fig.…”

Section: Resultsmentioning

confidence: 99%

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Structural and biochemical insights of CypA and AIF interaction

Farina

Sorbo

Chambery

et al. 2017

Sci Rep

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The Cyclophilin A (CypA)/Apoptosis Inducing Factor (AIF) complex is implicated in the DNA degradation in response to various cellular stress conditions, such as oxidative stress, cerebral hypoxia-ischemia and traumatic brain injury. The pro-apoptotic form of AIF (AIF(Δ1-121)) mainly interacts with CypA through the amino acid region 370–394. The AIF(370-394) synthetic peptide inhibits complex formation in vitro by binding to CypA and exerts neuroprotection in a model of glutamate-mediated oxidative stress. Here, the binding site of AIF(Δ1-121) and AIF(370-394) on CypA has been mapped by NMR spectroscopy and biochemical studies, and a molecular model of the complex has been proposed. We show that AIF(370-394) interacts with CypA on the same surface recognized by AIF(Δ1-121) protein and that the region is very close to the CypA catalytic pocket. Such region partially overlaps with the binding site of cyclosporin A (CsA), the strongest catalytic inhibitor of CypA. Our data point toward distinct CypA structural determinants governing the inhibitor selectivity and the differential biological effects of AIF and CsA, and provide new structural insights for designing CypA/AIF selective inhibitors with therapeutic relevance in neurodegenerative diseases.

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Section: Resultsmentioning

confidence: 99%

“…His-tagged CypA (hereafter CypA) and the corresponding R55A mutant, were expressed and purified as previously reported 25 . The protein concentration was determined by reading the absorbance at 280 nm with a NanoDrop200c UV-Vis spectrophotometer and using a theoretical molar extinction coefficient of 8730 M −1 cm −1 .…”

Section: Methodsmentioning

confidence: 99%

Structural and biochemical insights of CypA and AIF interaction

Farina

Sorbo

Chambery

et al. 2017

Sci Rep

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Small‐molecule inhibitors of cyclophilin D as potential therapeutics in mitochondria‐related diseases

Haleckova

Benek

Zemanová

et al. 2022

Medicinal Research Reviews

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Cyclophilin D (CypD) is a key regulator of mitochondrial permeability transition pore (mPTP) opening. This pathophysiological phenomenon is associated with the development of several human diseases, including ischemia‐reperfusion injury and neurodegeneration. Blocking mPTP opening through CypD inhibition could be a novel and promising therapeutic approach for these conditions. While numerous CypD inhibitors have been discovered to date, none have been introduced into clinical practice, mostly owing to their high toxicity, unfavorable pharmacokinetics, and low selectivity for CypD over other cyclophilins. This review summarizes current knowledge of CypD inhibitors, with a particular focus on small‐molecule compounds with regard to their in vitro activity, their selectivity for CypD, and their binding mode within the enzyme's active site. Finally, approaches for improving the molecular design of CypD inhibitors are discussed.

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Expression, Purification, Structural and Functional Characterization of Recombinant Human Parvulin 17

et al. 2022

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Parvulins, peptidyl-prolyl isomerase enzymes (PPIase), catalyze the cis–trans isomerization of prolyl bonds in polypeptides, contributing to folding and function regulation of many proteins. Among Parvulins, Par17, exclusively expressed in hominids, is the least examined in terms of structure, catalytic function and cellular activity. Setting the conditions for the preparation of recombinant active Par17 may therefore significantly foster future studies. Here, we comparatively evaluated the impact of several parameters, including host strains, culture media, isopropyl ß-D-1-thiogalactopyranoside concentration, post-induction incubation time and temperature, on the overexpression of Par17 in E. coli cells. A similar approach was also comparatively adopted for the preparation of the recombinant full-length Pin1 protein, the most representative Parvulin, and the catalytic domains of both enzymes. Proteins were efficiently expressed and purified to homogeneity and were subjected to a structural characterization by Size Exclusion Chromatography and Circular Dichroism. Moreover, a single-step homogeneous protease-based fluorimetric assay, potentially scalable in HTS format, has been developed for determining the peptidyl-prolyl cis–trans isomerase activity of recombinant Parvulins. Results obtained show that proteins are folded and active. These new data mark an important milestone for progressing the investigation of Parvulins.

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FRET-Protease-Coupled Peptidyl-Prolyl cis-trans Isomerase Assay

Cited by 7 publications

References 24 publications

Structural and biochemical insights of CypA and AIF interaction

Structural and biochemical insights of CypA and AIF interaction

Small‐molecule inhibitors of cyclophilin D as potential therapeutics in mitochondria‐related diseases

Expression, Purification, Structural and Functional Characterization of Recombinant Human Parvulin 17

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