Identification and characterization of the spiruchostatin biosynthetic gene cluster enable yield improvement by overexpressing a transcriptional activator

Author:

Potharla Vishwakanth Y12,Wang Cheng13,Cheng Yi-Qiang14

Affiliation:

1. grid.267468.9 0000000106957223 Department of Biological Sciences University of Wisconsin-Milwaukee PO Box 413 53201 Milwaukee WI USA

2. grid.30760.32 0000000121118460 Medical College of Wisconsin Milwaukee WI USA

3. Cedarburg Hauser Pharmaceuticals Grafton WI USA

4. grid.266871.c 0000000097656057 UNT System College of Pharmacy University of North Texas Health Science Center 3500 Camp Bowie Boulevard 76107 Fort Worth TX USA

Abstract

Abstract Spiruchostatins A and B are members of the FK228-family of natural products with potent histone deacetylase inhibitory activities and antineoplastic activities. However, their production in the wild-type strain of Pseudomonas sp. Q71576 is low. To improve the yield, the spiruchostatin biosynthetic gene cluster (spi) was first identified by rapid genome sequencing and characterized by genetic mutations. This spi gene cluster encodes a hybrid biosynthetic pathway similar to that encoded by the FK228 biosynthetic gene cluster (dep) in Chromobacterium violaceum No. 968. Each gene cluster contains a pathway regulatory gene (spiR vs. depR), but these two genes encode transcriptional activators of different classes. Overexpression of native spiR or heterologous depR in the wild-type strain of Pseudomonas sp. Q71576 resulted in 268 or 1,285 % increase of the combined titer of spiruchostatins A and B, respectively. RT-PCR analysis indicates that overexpression of heterologous depR upregulates the expression of native spiR.

Publisher

Oxford University Press (OUP)

Subject

Applied Microbiology and Biotechnology,Biotechnology,Bioengineering

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