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Molecular genetics and biochemistry of N-acetyltaurine degradation by Cupriavidus necator H16
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Cupriavidus necator H16 (DSM 428), whose genome has been sequenced, was found to degrade N-acetyltaurine as a sole source of carbon and energy for growth. Utilization of the compound was quantitative. The degradative pathway involved an inducible N-acetyltaurine amidohydrolase (NaaS), which catalysed the cleavage of N-acetyltaurine to acetate and taurine. The degradation of the latter compound is via an inducible, degradative pathway that involves taurine dehydrogenase [EC 1.4.2.–], sulfoacetaldehyde acetyltransferase [EC 2.3.3.15], phosphotransacetylase [EC 2.4.1.8], a sulfite exporter [TC 9.A.29.2.1] and sulfite dehydrogenase [EC 1.8.2.1]. Induction of the expression of representative gene products, encoded by at least four gene clusters, was confirmed biochemically. The acetate released by NaaS was activated to acetyl-CoA by an inducible acetate–CoA ligase [EC 6.2.1.1]. NaaS was purified to homogeneity; it had a K
m value of 9.4 mM for N-acetyltaurine, and it contained tightly bound Zn and Fe atoms. The denatured enzyme has a molecular mass of about 61 kDa (determined by SDS-PAGE) and the native enzyme was apparently monomeric. Peptide-mass fingerprinting identified the locus tag as H16_B0868 in a five-gene cluster, naaROPST (H16_B0865–H16_B0869). The cluster presumably encodes a LysR-type transcriptional regulator (NaaR), a membrane protein (NaaO), a solute : sodium symporter-family permease [TC 2.A.21] (NaaP), the metal-dependent amidohydrolase (NaaS) and a putative metallochaperone (COG0523) (NaaT). Reverse-transcription PCR indicated that naaOPST were inducibly transcribed.
Title: Molecular genetics and biochemistry of N-acetyltaurine degradation by Cupriavidus necator H16
Description:
Cupriavidus necator H16 (DSM 428), whose genome has been sequenced, was found to degrade N-acetyltaurine as a sole source of carbon and energy for growth.
Utilization of the compound was quantitative.
The degradative pathway involved an inducible N-acetyltaurine amidohydrolase (NaaS), which catalysed the cleavage of N-acetyltaurine to acetate and taurine.
The degradation of the latter compound is via an inducible, degradative pathway that involves taurine dehydrogenase [EC 1.
4.
2.
–], sulfoacetaldehyde acetyltransferase [EC 2.
3.
3.
15], phosphotransacetylase [EC 2.
4.
1.
8], a sulfite exporter [TC 9.
A.
29.
2.
1] and sulfite dehydrogenase [EC 1.
8.
2.
1].
Induction of the expression of representative gene products, encoded by at least four gene clusters, was confirmed biochemically.
The acetate released by NaaS was activated to acetyl-CoA by an inducible acetate–CoA ligase [EC 6.
2.
1.
1].
NaaS was purified to homogeneity; it had a K
m value of 9.
4 mM for N-acetyltaurine, and it contained tightly bound Zn and Fe atoms.
The denatured enzyme has a molecular mass of about 61 kDa (determined by SDS-PAGE) and the native enzyme was apparently monomeric.
Peptide-mass fingerprinting identified the locus tag as H16_B0868 in a five-gene cluster, naaROPST (H16_B0865–H16_B0869).
The cluster presumably encodes a LysR-type transcriptional regulator (NaaR), a membrane protein (NaaO), a solute : sodium symporter-family permease [TC 2.
A.
21] (NaaP), the metal-dependent amidohydrolase (NaaS) and a putative metallochaperone (COG0523) (NaaT).
Reverse-transcription PCR indicated that naaOPST were inducibly transcribed.
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