Your search keyword '"Jackson P. Jenkins"' showing total 3 results

1. Synthetic microbial communities of heterotrophs and phototrophs facilitate sustainable growth

Author

Cristal Zuñiga, Tingting Li, Michael T. Guarnieri, Jackson P. Jenkins, Chien-Ting Li, Kerem Bingol, Young-Mo Kim, Michael J. Betenbaugh, and Karsten Zengler

Subjects

Science

Abstract

Successful application of microbial community for bioproduction relies on the selection of appropriate heterotroph and phototroph partners. Here, the authors construct community metabolic models to guide strain selection and experimentally validate metabolic exchanges that sustain the heterotrophs in minimal media.

Published

2020

2. Mixed and membrane-separated culturing of synthetic cyanobacteria-yeast consortia reveals metabolic cross-talk mimicking natural cyanolichens

Author

Pavlo Bohutskyi, Kyle R. Pomraning, Jackson P Jenkins, Young-Mo Kim, Brenton C Poirier, Michael J Betenbaugh, and Jon K Magnuson

Subjects

Synthetic lichen, Microbial community, Membrane-separated bioreactor, Metabolite exchange, Phototroph-heterotroph co-culture, Cross-feeding, Medicine, Science

Abstract

Abstract Metabolite exchange mediates crucial interactions in microbial communities, significantly impacting global carbon and nitrogen cycling. Understanding these chemically-mediated interactions is essential for elucidating natural community functions and developing engineered synthetic communities. This study investigated membrane-separated bioreactors (mBRs) as a novel tool to identify transient metabolites and their producers/consumers in mixed microbial communities. We compared three co-culture methods (direct mixed, 2-chamber mBR, and 3-chamber mBR) to grow a synthetic binary community of the cyanobacterium Synechococcus elongatus PCC 7942 and the fungus Rhodotorula toruloides NBRC 0880, as well as axenic S. elongatus. Despite not being natural lichen constituents, these organisms exhibited interactions resembling those in cyanolichens. S. elongatus fixed CO2 into sugars as the primary shared metabolite, while R. toruloides secreted various biochemicals, predominantly sugar alcohols, mirroring the metabolite exchange observed in natural lichens. The mBR systems successfully captured metabolite gradients and revealed rapidly consumed compounds, including TCA cycle intermediates and amino acids. Our approach demonstrated that the 2-chamber mBR optimally balanced metabolite exchange and growth dynamics. This study provides insights into cross-species metabolic interactions and presents a valuable tool for investigating and engineering synthetic microbial communities with potential applications in biotechnology and environmental science.

Published

2024

3. One Primer To Rule Them All: Universal Primer That Adds BBa_B0034 Ribosomal Binding Site to Any Coding Standard 10 BioBrick

Author

Vincent F. Fiore, Jackson P Jenkins, Haoli Du, Tilak Balavijayan, Rachael M Blackstone, Casey L Haynes, Anton V. Bryksin, Jessica L Siemer, Spencer W. Cooper, Thomas H. Barker, and Haylee Bachman

Subjects

Genetics, Binding Sites, Extramural, Biomedical Engineering, General Medicine, Biology, BioBrick, Biochemistry, Genetics and Molecular Biology (miscellaneous), Ribosome, Ribosomal binding site, Viewpoint, Mutagenesis, Site-Directed, Primer (molecular biology), Molecular Biology, Ribosomes, DNA Primers, Plasmids

Abstract

Here, we present a universal, simple, efficient, and reliable way to add small BioBrick parts to any BioBrick via PCR that is compatible with BioBrick assembly standard 10. As a proof of principle, we have designed a universal primer, rbs_B0034, that contains a ribosomal binding site (RBS; BBa_B0034) and that can be used in PCR to amplify any coding BioBrick that starts with ATG. We performed test PCRs with rbs_B0034 on 31 different targets and found it to be 93.6% efficient. Moreover, when supplemented with a complementary primer, addition of RBS can be accomplished via whole plasmid site-directed mutagenesis, thus reducing the time required for further assembly of composite parts. The described method brings simplicity to the addition of small parts, such as regulatory elements to existing BioBricks. The final product of the PCR assembly is indistinguishable from the standard or 3A BioBrick assembly.

Published

2014