AUTHOR=Ujor Victor Chinomso , Lai Lien B. , Okonkwo Christopher Chukwudi , Gopalan Venkat , Ezeji Thaddeus Chukwuemeka 

TITLE=Ribozyme-Mediated Downregulation Uncovers DNA Integrity Scanning Protein A (DisA) as a Solventogenesis Determinant in Clostridium beijerinckii

JOURNAL=Frontiers in Bioengineering and Biotechnology

VOLUME=9

YEAR=2021

URL=https://www.frontiersin.org/journals/bioengineering-and-biotechnology/articles/10.3389/fbioe.2021.669462

DOI=10.3389/fbioe.2021.669462

ISSN=2296-4185

ABSTRACT=<p>Carbon catabolite repression (CCR) limits microbial utilization of lignocellulose-derived pentoses. To relieve CCR in <italic>Clostridium beijerinckii</italic> NCIMB 8052, we sought to downregulate catabolite control protein A (CcpA) using the M1GS ribozyme technology. A CcpA-specific ribozyme was constructed by tethering the catalytic subunit of <italic>Escherichia coli</italic> RNase P (M1 RNA) to a guide sequence (GS) targeting CcpA mRNA (M1GS<sup>CcpA</sup>). As negative controls, the ribozyme M1GS<sup>CcpA–Sc</sup> (constructed with a scrambled GS<sup>CcpA</sup>) or the empty plasmid pMTL500E were used. With a ∼3-fold knockdown of CcpA mRNA in <italic>C. beijerinckii</italic> expressing M1GS<sup>CcpA</sup> (<italic>C. beijerinckii</italic>_M1GS<sup>CcpA</sup>) relative to both controls, a modest enhancement in mixed-sugar utilization and solvent production was achieved. Unexpectedly, <italic>C. beijerinckii</italic>_M1GS<sup>CcpA–Sc</sup> produced 50% more solvent than <italic>C. beijerinckii</italic>_pMTL500E grown on glucose + arabinose. Sequence complementarity (albeit suboptimal) suggested that M1GS<sup>CcpA–Sc</sup> could target the mRNA encoding DNA integrity scanning protein A (DisA), an expectation that was confirmed by a 53-fold knockdown in DisA mRNA levels. Therefore, M1GS<sup>CcpA–Sc</sup> was renamed M1GS<sup>DisA</sup>. Compared to <italic>C. beijerinckii</italic>_M1GS<sup>CcpA</sup> and _pMTL500E, <italic>C. beijerinckii</italic>_M1GS<sup>DisA</sup> exhibited a 7-fold decrease in the intracellular c-di-AMP level after 24 h of growth and a near-complete loss of viability upon exposure to DNA-damaging antibiotics. Alterations in c-di-AMP-mediated signaling and cell cycling likely culminate in a sporulation delay and the solvent production gains observed in <italic>C. beijerinckii</italic>_M1GS<sup>DisA</sup>. Successful knockdown of the CcpA and DisA mRNAs demonstrate the feasibility of using M1GS technology as a metabolic engineering tool for increasing butanol production in <italic>C. beijerinckii</italic>.</p>