Genetic characterization of enzymes involved in the priming steps of oxytetracycline biosynthesis in Streptomyces rimosus

Tetracyclines are clinically important aromatic polyketides whose biosynthesis is catalysed by bacterial type II polyketide synthases (PKSs). Tetracyclines are biosynthesized starting with an amide-containing malonamate starter unit and the resulting C-2 carboxyamide is critical for the antibiotic a...

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Veröffentlicht in:	Microbiology (Society for General Microbiology) 2011-08, Vol.157 (Pt 8), p.2401-2409
Hauptverfasser:	PENGWANG, XUE GAO, CHOOI, Yit-Heng, ZIXINDENG, YITANG
Format:	Artikel
Sprache:	eng
Schlagworte:	Anti-Bacterial Agents - biosynthesis Bacterial Proteins - chemistry Bacterial Proteins - genetics Bacteriology Biological and medical sciences Biosynthetic Pathways Enzymes - chemistry Enzymes - genetics Fundamental and applied biological sciences. Psychology Gene Knockout Techniques Genetic Complementation Test Microbiology Miscellaneous Models, Biological Models, Molecular Mutation, Missense Oxytetracycline - biosynthesis Streptomyces - genetics Streptomyces - metabolism Streptomyces rimosus
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container_end_page	2409
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container_title	Microbiology (Society for General Microbiology)
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creator	PENGWANG XUE GAO CHOOI, Yit-Heng ZIXINDENG YITANG
description	Tetracyclines are clinically important aromatic polyketides whose biosynthesis is catalysed by bacterial type II polyketide synthases (PKSs). Tetracyclines are biosynthesized starting with an amide-containing malonamate starter unit and the resulting C-2 carboxyamide is critical for the antibiotic activities. In this work, we genetically verified that an amidotransferase, OxyD, and a thiolase, OxyP, are involved in the biosynthesis and incorporation of the starter unit. First, two mutations, R248T and D268N, were found to be present in OxyD* encoded in Streptomyces rimosus ATCC 13224, a strain that produces the acetate-primed 2-acetyl-2-decarboxyamido-oxytetracycline (ADOTC) instead of the malonamate-primed oxytetracycline (OTC). Homology modelling suggested that in particular D268N may inactivate OxyD. Complementation of S. rimosus ATCC 13224 with wild-type OxyD restored OTC biosynthesis, thereby confirming the essential role of OxyD in the synthesis of the amide starter unit. Second, using a series of knockout and complementation approaches, we demonstrated that OxyP is most likely involved in maintaining fidelity of the amide-priming process via hydrolysis of the competing acetate priming starter units. While the inactivation of OxyP does not eliminate OTC biosynthesis, the ratio of acetate-primed ADOTC to malonamate-primed OTC is significantly increased. This suggests that OxyP plays an ancillary role in OTC biosynthesis and is important for minimizing the levels of ADOTC, a shunt product that has much weaker antibiotic activities than OTC.
doi_str_mv	10.1099/mic.0.048439-0
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Tetracyclines are biosynthesized starting with an amide-containing malonamate starter unit and the resulting C-2 carboxyamide is critical for the antibiotic activities. In this work, we genetically verified that an amidotransferase, OxyD, and a thiolase, OxyP, are involved in the biosynthesis and incorporation of the starter unit. First, two mutations, R248T and D268N, were found to be present in OxyD* encoded in Streptomyces rimosus ATCC 13224, a strain that produces the acetate-primed 2-acetyl-2-decarboxyamido-oxytetracycline (ADOTC) instead of the malonamate-primed oxytetracycline (OTC). Homology modelling suggested that in particular D268N may inactivate OxyD. Complementation of S. rimosus ATCC 13224 with wild-type OxyD restored OTC biosynthesis, thereby confirming the essential role of OxyD in the synthesis of the amide starter unit. Second, using a series of knockout and complementation approaches, we demonstrated that OxyP is most likely involved in maintaining fidelity of the amide-priming process via hydrolysis of the competing acetate priming starter units. While the inactivation of OxyP does not eliminate OTC biosynthesis, the ratio of acetate-primed ADOTC to malonamate-primed OTC is significantly increased. 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Second, using a series of knockout and complementation approaches, we demonstrated that OxyP is most likely involved in maintaining fidelity of the amide-priming process via hydrolysis of the competing acetate priming starter units. While the inactivation of OxyP does not eliminate OTC biosynthesis, the ratio of acetate-primed ADOTC to malonamate-primed OTC is significantly increased. This suggests that OxyP plays an ancillary role in OTC biosynthesis and is important for minimizing the levels of ADOTC, a shunt product that has much weaker antibiotic activities than OTC.</description><subject>Anti-Bacterial Agents - biosynthesis</subject><subject>Bacterial Proteins - chemistry</subject><subject>Bacterial Proteins - genetics</subject><subject>Bacteriology</subject><subject>Biological and medical sciences</subject><subject>Biosynthetic Pathways</subject><subject>Enzymes - chemistry</subject><subject>Enzymes - genetics</subject><subject>Fundamental and applied biological sciences. 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subjects	Anti-Bacterial Agents - biosynthesis Bacterial Proteins - chemistry Bacterial Proteins - genetics Bacteriology Biological and medical sciences Biosynthetic Pathways Enzymes - chemistry Enzymes - genetics Fundamental and applied biological sciences. Psychology Gene Knockout Techniques Genetic Complementation Test Microbiology Miscellaneous Models, Biological Models, Molecular Mutation, Missense Oxytetracycline - biosynthesis Streptomyces - genetics Streptomyces - metabolism Streptomyces rimosus
title	Genetic characterization of enzymes involved in the priming steps of oxytetracycline biosynthesis in Streptomyces rimosus
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