Unnatural amino acids increase activity and specificity of synthetic substrates for human and malarial cathepsin C

Poręba, Marcin; Mihelič, Marko; Krai, Priscilla; Rajkovic, Jelena; Krężel, Artur; Pawełczak, Małgorzata; Klemba, Michael; Turk, Dušan; Turk, Boris; Latajka, Rafał; Drąg, Marcin

doi:10.1007/s00726-013-1654-2

Cited by 37 publications

(54 citation statements)

References 25 publications

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“…2). This result was apparently not in agreement with the previously reported experimental results concerning the inhibitory effects of D amino acids or their unnat ural derivatives on cysteine, serine and aspartic types of proteases [13][14][15][16][17]. It might have 2 explanations as follows: 1-D amino acids do not interact with the fusion form of CP/CPI pair, or 2-D amino acids interact with the fusion form of CP/CPI pair in a man ner that does not affect the functionality of R1 prod uct.…”

Section: Resultscontrasting

confidence: 72%

“…To date, the develop ment and the use of efficient synthetic proteinase inhibitors including various non natural D amino acid derivatives are the most challenging task and tool to prevent their pathogenicities, in vivo [13,14]. In a recent study, the activity and the specificity of syn thetic peptides containing unnatural amino acids have been reported to be increased for human and malarial cysteine proteinases [17].…”

mentioning

confidence: 99%

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Differential effects of D-amino acids on the fusion forms of a cysteine proteinase/cystatin pair

Gholizadeh

2015

Appl Biochem Microbiol

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The interactions of 2 different fusion constructs of a plant cysteine proteinase (CP)/cysteine protein ase inhibitor (CPI) pair designated as R1: H 2 N maltose binding protein CPI CP COOH and R2: H 2 N mal tose binding protein CP CPI COOH with 4 different D amino acids including D Ala, D Ser, D Asp and D Phe were analyzed using experimental methods and computational tools. The results showed that the relative activity of CP is increased in purified R2 product and test D amino acids tend to interact with CP/CPI pair. In contrast, the functionality of R1 product was not influenced by test D amino acids. Determination of the effects of D enantiomers of amino acids on the fusion forms of 2 functionally related proteins such as CP and CPI is the first research in this area. The results related to the binding abilities and the functional properties of 2 differ entially organized forms of CP/CPI pair are predicted to be used as biotechnological clues to make switchable expression systems of 2 functionally related proteins in the future.

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Section: Resultscontrasting

confidence: 72%

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confidence: 99%

Differential effects of D-amino acids on the fusion forms of a cysteine proteinase/cystatin pair

Gholizadeh

2015

Appl Biochem Microbiol

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“…In this manner, the sets of data that may be useful for design and synthesis of selective inhibitors are obtained (Drąg et al 2010;Kasperkiewicz et al 2012;Poras et al 2011Poras et al , 2013Węglarz-Tomczak et al 2013;Poręba et al 2014).…”

Section: Introductionmentioning

confidence: 99%

The influence of α-aminophosphonic acids on the activity of aminopeptidase from barley seeds—an approach to determine the enzyme specificity

2015

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Inhibitory potencies of 24 a-aminophosphonic acids against barley seeds (Hordeum vulgare L.) metalloaminopeptidase have been determined to evaluate structural requirements of this enzyme. The enzyme was sensitive mostly to the influence of phosphonic acid analogues of phenylalanine and its homologues, thus showing narrow specificity if compared with porcine aminopeptidases M1 and M17 and with Plasmodium aminopeptidase M17.

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“…The heat map shown in Fig. B compares the specificities of DPAP3 with those previously obtained for DPAP1 and CatC at the same substrate concentration. Note that D ‐Phg is the only D‐ AA in P2 that is cleaved by DPAP3, albeit poorly.…”

Section: Resultsmentioning

confidence: 78%

“… For DPAP1, k cat = 0.22 ± 0.004 s −1 , K m = 0.67 ± 0.14 μ m and k cat / K m = 320 000 ± 50 000 m −1 ·s −1 ; for CatC, k cat = 10.8 ± 0.2 s −1 , K m = 91 ± 5 μ m and k cat / K m = 116 000 ± 11 000 m −1 ·s −1 . …”

Section: Resultsmentioning

confidence: 95%

Characterization of P. falciparum dipeptidyl aminopeptidase 3 specificity identifies differences in amino acid preferences between peptide‐based substrates and covalent inhibitors

et al. 2019

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Malarial dipeptidyl aminopeptidases (DPAPs) are cysteine proteases important for parasite development thus making them attractive drug targets. In order to develop inhibitors specific to the parasite enzymes, it is necessary to map the determinants of substrate specificity of the parasite enzymes and its mammalian homologue cathepsin C (CatC). Here, we screened peptide‐based libraries of substrates and covalent inhibitors to characterize the differences in specificity between parasite DPAPs and CatC, and used this information to develop highly selective DPAP1 and DPAP3 inhibitors. Interestingly, while the primary amino acid specificity of a protease is often used to develop potent inhibitors, we show that equally potent and highly specific inhibitors can be developed based on the sequences of nonoptimal peptide substrates. Finally, our homology modelling and docking studies provide potential structural explanations of the differences in specificity between DPAP1, DPAP3, and CatC, and between substrates and inhibitors in the case of DPAP3. Overall, this study illustrates that focusing the development of protease inhibitors solely on substrate specificity might overlook important structural features that can be exploited to develop highly potent and selective compounds.

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Unnatural amino acids increase activity and specificity of synthetic substrates for human and malarial cathepsin C

Cited by 37 publications

References 25 publications

Differential effects of D-amino acids on the fusion forms of a cysteine proteinase/cystatin pair

Differential effects of D-amino acids on the fusion forms of a cysteine proteinase/cystatin pair

The influence of α-aminophosphonic acids on the activity of aminopeptidase from barley seeds—an approach to determine the enzyme specificity

Characterization of P. falciparum dipeptidyl aminopeptidase 3 specificity identifies differences in amino acid preferences between peptide‐based substrates and covalent inhibitors

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