High-level expression of codon-optimized Taq DNA polymerase under the control of rhaBAD promoter.

Laksmi, Fina Amreta; Dewi, Kartika Sari; Nuryana, Isa; Yulianti, Siti Eka; Ramadhan, Kharisma Panji; Hadi, Moch Irfan; Nugraha, Yudhi

Laksmi, Fina Amreta; Dewi, Kartika Sari; Nuryana, Isa; Yulianti, Siti Eka; Ramadhan, Kharisma Panji; Hadi, Moch Irfan; Nugraha, Yudhi.

Afiliación

Laksmi FA; Research Center for Applied Microbiology, National Research and Innovation Agency, Jalan Raya Bogor KM 46, Cibinong, Bogor, 16911, West Java, Indonesia. Electronic address: fina003@brin.go.id.
Dewi KS; Research Center for Genetic Engineering, National Research and Innovation Agency, Jalan Raya Bogor KM 46, Cibinong, Bogor, 16911, West Java, Indonesia.
Nuryana I; Research Center for Applied Microbiology, National Research and Innovation Agency, Jalan Raya Bogor KM 46, Cibinong, Bogor, 16911, West Java, Indonesia.
Yulianti SE; Research Center for Applied Microbiology, National Research and Innovation Agency, Jalan Raya Bogor KM 46, Cibinong, Bogor, 16911, West Java, Indonesia.
Ramadhan KP; Research Center for Applied Microbiology, National Research and Innovation Agency, Jalan Raya Bogor KM 46, Cibinong, Bogor, 16911, West Java, Indonesia.
Hadi MI; Department of Biology, Sunan Ampel State Islamic University, Surabaya, Indonesia.
Nugraha Y; Research Center for Molecular Biology Eijkman, National Research and Innovation Agency, Jalan Raya Bogor KM 46, Cibinong, Bogor, 16911, West Java, Indonesia. Electronic address: yudhi.nugraha@brin.go.id.

Anal Biochem ; 692: 115581, 2024 Sep.

Article en En | MEDLINE | ID: mdl-38815728

ABSTRACT

ABSTRACT

A DNA polymerase from Thermus aquaticus remains the most popular among DNA polymerases. It was widely applied in various fields involving the application of polymerase chain reaction (PCR), implying the high commercial value of this enzyme. For this reason, an attempt to obtain a high yield of Taq DNA polymerase is continuously conducted. In this study, the l-rhamnose-inducible promoter rhaBAD was utilized due to its ability to produce recombinant protein under tight control in E. coli expression system. Instead of full-length Taq polymerase, an N-terminal deletion of Taq polymerase was selected. To obtain a high-level expression, we attempted to optimize the codon by reducing the rare codon and GC content, and in a second attempt, we optimized the culture conditions for protein expression. The production of Taq polymerase using the optimum culture condition improved the level of expression by up to 3-fold. This approach further proved that a high level of recombinant protein expression could be achieved by yielding a purified Taq polymerase of about 8.5 mg/L of culture. This is the first research publication on the production of Taq polymerase with N-terminal deletion in E. coli with the control of the rhaBAD promoter system.

Asunto(s)

Codón; Escherichia coli; Regiones Promotoras Genéticas; Proteínas Recombinantes; Polimerasa Taq; Escherichia coli/genética; Escherichia coli/metabolismo; Codón/genética; Polimerasa Taq/metabolismo; Polimerasa Taq/genética; Proteínas Recombinantes/genética; Proteínas Recombinantes/biosíntesis; Proteínas Recombinantes/metabolismo; Thermus/genética; Thermus/enzimología; Secuencia de Bases

Palabras clave

Escherichia coli; Taq polymerase; codon optimization; culture conditions; rhaBAD promoter

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Texto completo: 1 Colección: 01-internacional Base de datos: MEDLINE Asunto principal: Proteínas Recombinantes / Codón / Regiones Promotoras Genéticas / Polimerasa Taq / Escherichia coli Idioma: En Revista: Anal Biochem Año: 2024 Tipo del documento: Article Pais de publicación: Estados Unidos

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