Literature summary extracted from

Cui, Y.; Cui, W.; Liu, Z.; Zhou, L.; Kobayashi, M.; Zhou, Z.
Improvement of stability of nitrile hydratase via protein fragment swapping (2014), Biochem. Biophys. Res. Commun., 450, 401-408.

Cloned(Commentary)

EC Number	Cloned (Comment)	Organism
4.2.1.84	genetic organization of wild-type and chimeric mutant enzymes, expression of wild-type and recombinant chimeric mutants in Escherichia coli strain JM109	Pseudomonas putida
4.2.1.84	genetic organization of wild-type and chimeric mutant enzymes, expression of wild-type and recombinant chimeric mutants in Escherichia coli strain JM109	Comamonas testosteroni
4.2.1.84	genetic organization of wild-type and chimeric mutant enzymes, expression of wild-type and recombinant chimeric mutants in Escherichia coli strain JM109	Pseudonocardia thermophila

Protein Variants

EC Number	Protein Variants	Comment	Organism
4.2.1.84	additional information	homologous protein fragment swapping method is used for the improvement of the stability of NHase from Pseudomonas putida NRRL-18668, site targeted amino recombination software and molecular dynamics are used for determination of the crossover sites for fragment recombination, overview. One thermophilic NHase fragment M1 to G98 from Comamonas testosteroni 5-MGAM-4D and two fragments K165-V196 and K165-D209 from Pseudonocardia thermophila JCM3095 are selected to swap the corresponding fragments of Pseudomonas putida NHase. The chimeric NHases show 1.4 to 3.5fold enhancement in thermostability, some show reduced activity and product inhibition compared to wild-type Pseudomonas putida NHase. But mutants 3AB and 3ABC show increased activity due to altered secondary structure compared to the Pseudomonas putida wild-type	Comamonas testosteroni
4.2.1.84	additional information	homologous protein fragment swapping method is used for the improvement of the stability of NHase from Pseudomonas putida NRRL-18668, site targeted amino recombination software and molecular dynamics are used for determination of the crossover sites for fragment recombination, overview. One thermophilic NHase fragment M1 to G98 from Comamonas testosteroni 5-MGAM-4D and two fragments K165-V196 and K165-D209 from Pseudonocardia thermophila JCM3095 are selected to swap the corresponding fragments of Pseudomonas putida NHase. The chimeric NHases show 1.4 to 3.5fold enhancement in thermostability, some show reduced activity and product inhibition compared to wild-type Pseudomonas putida NHase. But mutants 3AB and 3ABC show increased activity due to altered secondary structure compared to the Pseudomonas putida wild-type	Pseudonocardia thermophila
4.2.1.84	additional information	homologous protein fragment swapping method is used for the improvement of the stability of NHase from Pseudomonas putida NRRL-18668, site targeted amino recombination software and molecular dynamics are used for determination of the crossover sites for fragment recombination, overview. One thermophilic NHase fragment M1 to G98 from Comamonas testosteroni 5-MGAM-4D and two fragments K165-V196 and K165-D209 from Pseudonocardia thermophila JCM3095 are selected to swap the corresponding fragments of Pseudomonas putida NHase. The chimeric NHases show 1.4 to 3.5fold enhancement in thermostability, some show reduced activity and product inhibition compared to wild-type Pseudomonas putida NHase. But mutants 3AB and 3ABC show increased activity due to altered secondary structure compared to the wild-type	Pseudomonas putida

Inhibitors

EC Number	Inhibitors	Comment	Organism	Structure
4.2.1.84	additional information	product inhibition at high concentrations	Pseudomonas putida

Organism

EC Number	Organism	UniProt	Comment	Textmining
4.2.1.84	Comamonas testosteroni	Q5XPL4	beta subunit	-
4.2.1.84	Comamonas testosteroni	Q5XPL5	alpha subunit	-
4.2.1.84	Comamonas testosteroni 5-MGAM-4D	Q5XPL4	beta subunit	-
4.2.1.84	Comamonas testosteroni 5-MGAM-4D	Q5XPL5	alpha subunit	-
4.2.1.84	Pseudomonas putida	-	-	-
4.2.1.84	Pseudomonas putida NRRL-18668	-	-	-
4.2.1.84	Pseudonocardia thermophila	Q7SID2	alpha-subunit	-
4.2.1.84	Pseudonocardia thermophila	Q7SID3	beta-subunit	-
4.2.1.84	Pseudonocardia thermophila JCM 3095	Q7SID2	alpha-subunit	-
4.2.1.84	Pseudonocardia thermophila JCM 3095	Q7SID3	beta-subunit	-

Specific Activity [micromol/min/mg]

EC Number	Specific Activity Minimum [µmol/min/mg]	Specific Activity Maximum [µmol/min/mg]	Comment	Organism
4.2.1.84	439	-	purified recombinant wild-type enzyme, pH 7.5, 20°C	Pseudomonas putida
4.2.1.84	483	-	purified recombinant chimeric mutant 3ABC, pH 7.5, 20°C	Pseudomonas putida
4.2.1.84	614	-	purified recombinant chimeric mutant 3AB, pH 7.5, 20°C	Pseudomonas putida

Substrates and Products (Substrate)

EC Number	Substrates	Comment Substrates	Organism	Products	Comment (Products)	Rev.	Reac.
4.2.1.84	3-cyanopyridine + H2O	-	Pseudomonas putida	pyridine-3-carbamide	-	?
4.2.1.84	3-cyanopyridine + H2O	-	Comamonas testosteroni	pyridine-3-carbamide	-	?
4.2.1.84	3-cyanopyridine + H2O	-	Pseudonocardia thermophila	pyridine-3-carbamide	-	?
4.2.1.84	3-cyanopyridine + H2O	-	Comamonas testosteroni 5-MGAM-4D	pyridine-3-carbamide	-	?
4.2.1.84	3-cyanopyridine + H2O	-	Pseudomonas putida NRRL-18668	pyridine-3-carbamide	-	?
4.2.1.84	3-cyanopyridine + H2O	-	Pseudonocardia thermophila JCM 3095	pyridine-3-carbamide	-	?

Synonyms

EC Number	Synonyms	Comment	Organism
4.2.1.84	NHase	-	Pseudomonas putida
4.2.1.84	NHase	-	Comamonas testosteroni
4.2.1.84	NHase	-	Pseudonocardia thermophila

Temperature Optimum [°C]

EC Number	Temperature Optimum [°C]	Temperature Optimum Maximum [°C]	Comment	Organism
4.2.1.84	20	-	assay at	Pseudomonas putida
4.2.1.84	20	-	assay at	Comamonas testosteroni
4.2.1.84	20	-	assay at	Pseudonocardia thermophila

pH Optimum

EC Number	pH Optimum Minimum	pH Optimum Maximum	Comment	Organism
4.2.1.84	7.5	-	assay at	Pseudomonas putida
4.2.1.84	7.5	-	assay at	Comamonas testosteroni
4.2.1.84	7.5	-	assay at	Pseudonocardia thermophila

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Release 2023.1 (January 2023)