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2. Gene Editing/Gene Therapies: HOMOLOGY-INDEPENDENT TARGETED INSERTION (HITI) ENABLES GUIDED CAR KNOCK-IN AND EFFICIENT CLINICAL SCALE CAR-T CELL MANUFACTURING

Author

Balke-Want, H., primary, Keerthi, V., additional, Gkitsas, N., additional, Mancini, A., additional, Kurgan, G., additional, Fowler, C., additional, Xu, P., additional, Liu, X., additional, Asano, K., additional, Patel, S., additional, Fisher, C., additional, Brown, A., additional, Tunuguntla, R., additional, Sotillo, E., additional, Mackall, C., additional, and Feldman, S., additional

Published
2023
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5. Shuttle peptide delivers base editor RNPs to rhesus monkey airway epithelial cells in vivo.

Author

Kulhankova K, Traore S, Cheng X, Benk-Fortin H, Hallée S, Harvey M, Roberge J, Couture F, Kohli S, Gross TJ, Meyerholz DK, Rettig GR, Thommandru B, Kurgan G, Wohlford-Lenane C, Hartigan-O'Connor DJ, Yates BP, Newby GA, Liu DR, Tarantal AF, Guay D, and McCray PB Jr

Subjects
Animals, Humans, Mice, Macaca mulatta metabolism, Respiratory Mucosa metabolism, Ribonucleoproteins metabolism, Peptides genetics, CRISPR-Cas Systems, Cystic Fibrosis Transmembrane Conductance Regulator genetics, Cystic Fibrosis Transmembrane Conductance Regulator metabolism, Epithelial Cells metabolism
Abstract

Gene editing strategies for cystic fibrosis are challenged by the complex barrier properties of airway epithelia. We previously reported that the amphiphilic S10 shuttle peptide non-covalently combined with CRISPR-associated (Cas) ribonucleoprotein (RNP) enabled editing of human and mouse airway epithelial cells. Here, we derive the S315 peptide as an improvement over S10 in delivering base editor RNP. Following intratracheal aerosol delivery of Cy5-labeled peptide in rhesus macaques, we confirm delivery throughout the respiratory tract. Subsequently, we target CCR5 with co-administration of ABE8e-Cas9 RNP and S315. We achieve editing efficiencies of up-to 5.3% in rhesus airway epithelia. Moreover, we document persistence of edited epithelia for up to 12 months in mice. Finally, delivery of ABE8e-Cas9 targeting the CFTR R553X mutation restores anion channel function in cultured human airway epithelia. These results demonstrate the therapeutic potential of base editor delivery with S315 to functionally correct the CFTR R553X mutation in respiratory epithelia., (© 2023. The Author(s).)

Published
2023
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6. Directed evolution of Zymomonas mobilis sugar facilitator Glf to overcome glucose inhibition.

Author

Kurgan G, Onyeabor M, Holland SC, Taylor E, Schneider A, Kurgan L, Billings T, and Wang X

Subjects
Escherichia coli genetics, Fermentation, Glucose, Sugars, Xylose, Zymomonas genetics
Abstract

Cellular import of D-xylose, the second most abundant sugar in typical lignocellulosic biomass, has been evidenced to be an energy-depriving process in bacterial biocatalysts. The sugar facilitator of Zymomonas mobilis, Glf, is capable of importing xylose at high rates without extra energy input, but is inhibited by D-glucose (the primary biomass sugar), potentially limiting the utility of this transporter for fermentation of sugar mixtures derived from lignocellulose. In this work we developed an Escherichia coli platform strain deficient in glucose and xylose transport to facilitate directed evolution of Glf to overcome glucose inhibition. Using this platform, we isolated nine Glf variants created by both random and site-saturation mutagenesis with increased xylose utilization rates ranging from 4.8-fold to 13-fold relative to wild-type Glf when fermenting 100 g l-1 glucose-xylose mixtures. Diverse point mutations such as A165M and L445I were discovered leading to released glucose inhibition. Most of these mutations likely alter sugar coordinating pocket for the 6-hydroxymethyl group of D-glucose. These discovered glucose-resistant Glf variants can be potentially used as energy-conservative alternatives to the native sugar transport systems of bacterial biocatalysts for fermentation of lignocellulose-derived sugars., (© The Author(s) 2021. Published by Oxford University Press on behalf of Society of Industrial Microbiology and Biotechnology.)

Published
2022
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7. Efficiency, Specificity and Temperature Sensitivity of Cas9 and Cas12a RNPs for DNA-free Genome Editing in Plants.

Author

Banakar R, Schubert M, Kurgan G, Rai KM, Beaudoin SF, Collingwood MA, Vakulskas CA, Wang K, and Zhang F

Abstract

Delivery of genome editing reagents using CRISPR-Cas ribonucleoproteins (RNPs) transfection offers several advantages over plasmid DNA-based delivery methods, including reduced off-target editing effects, mitigation of random integration of non-native DNA fragments, independence of vector constructions, and less regulatory restrictions. Compared to the use in animal systems, RNP-mediated genome editing is still at the early development stage in plants. In this study, we established an efficient and simplified protoplast-based genome editing platform for CRISPR-Cas RNP delivery, and then evaluated the efficiency, specificity, and temperature sensitivity of six Cas9 and Cas12a proteins. Our results demonstrated that Cas9 and Cas12a RNP delivery resulted in genome editing frequencies (8.7-41.2%) at various temperature conditions, 22°C, 26°C, and 37°C, with no significant temperature sensitivity. LbCas12a often exhibited the highest activities, while AsCas12a demonstrated higher sequence specificity. The high activities of CRISPR-Cas RNPs at 22° and 26°C, the temperature preferred by plant transformation and tissue culture, led to high mutagenesis efficiencies (34.0-85.2%) in the protoplast-regenerated calli and plants with the heritable mutants recovered in the next generation. This RNP delivery approach was further extended to pennycress ( Thlaspi arvense ), soybean ( Glycine max ) and Setaria viridis with up to 70.2% mutagenesis frequency. Together, this study sheds light on the choice of RNP reagents to achieve efficient transgene-free genome editing in plants., Competing Interests: MS, GK, SB, MC, and CV was employed by the company Integrated DNA Technologies. The remaining authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2022 Banakar, Schubert, Kurgan, Rai, Beaudoin, Collingwood, Vakulskas, Wang and Zhang.)

Published
2022
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8. Optimized design parameters for CRISPR Cas9 and Cas12a homology-directed repair.

Author

Schubert MS, Thommandru B, Woodley J, Turk R, Yan S, Kurgan G, McNeill MS, and Rettig GR

Subjects
Cell Line, Humans, Mutation, RNA, Guide, CRISPR-Cas Systems genetics, Bacterial Proteins metabolism, CRISPR-Associated Protein 9 metabolism, CRISPR-Associated Proteins metabolism, CRISPR-Cas Systems, Endodeoxyribonucleases metabolism, Gene Editing, Recombinational DNA Repair
Abstract

CRISPR-Cas proteins are RNA-guided nucleases used to introduce double-stranded breaks (DSBs) at targeted genomic loci. DSBs are repaired by endogenous cellular pathways such as non-homologous end joining (NHEJ) and homology-directed repair (HDR). Providing an exogenous DNA template during repair allows for the intentional, precise incorporation of a desired mutation via the HDR pathway. However, rates of repair by HDR are often slow compared to the more rapid but less accurate NHEJ-mediated repair. Here, we describe comprehensive design considerations and optimized methods for highly efficient HDR using single-stranded oligodeoxynucleotide (ssODN) donor templates for several CRISPR-Cas systems including S.p. Cas9, S.p. Cas9 D10A nickase, and A.s. Cas12a delivered as ribonucleoprotein (RNP) complexes. Features relating to guide RNA selection, donor strand preference, and incorporation of blocking mutations in the donor template to prevent re-cleavage were investigated and were implemented in a novel online tool for HDR donor template design. These findings allow for high frequencies of precise repair utilizing HDR in multiple mammalian cell lines. Tool availability: https://www.idtdna.com/HDR., (© 2021. The Author(s).)

Published
2021
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9. CRISPECTOR provides accurate estimation of genome editing translocation and off-target activity from comparative NGS data.

Author

Amit I, Iancu O, Levy-Jurgenson A, Kurgan G, McNeill MS, Rettig GR, Allen D, Breier D, Ben Haim N, Wang Y, Anavy L, Hendel A, and Yakhini Z

Subjects
Algorithms, DNA-Binding Proteins genetics, HEK293 Cells, Homeodomain Proteins genetics, Humans, Nuclear Proteins genetics, Software, Transcription Factors genetics, CRISPR-Cas Systems, Computational Biology methods, Gene Editing methods
Abstract

Controlling off-target editing activity is one of the central challenges in making CRISPR technology accurate and applicable in medical practice. Current algorithms for analyzing off-target activity do not provide statistical quantification, are not sufficiently sensitive in separating signal from noise in experiments with low editing rates, and do not address the detection of translocations. Here we present CRISPECTOR, a software tool that supports the detection and quantification of on- and off-target genome-editing activity from NGS data using paired treatment/control CRISPR experiments. In particular, CRISPECTOR facilitates the statistical analysis of NGS data from multiplex-PCR comparative experiments to detect and quantify adverse translocation events. We validate the observed results and show independent evidence of the occurrence of translocations in human cell lines, after genome editing. Our methodology is based on a statistical model comparison approach leading to better false-negative rates in sites with weak yet significant off-target activity.

Published
2021
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10. Characterizing Escherichia coli's transcriptional response to different styrene exposure modes reveals novel toxicity and tolerance insights.

Author

Machas M, Kurgan G, Abed OA, Shapiro A, Wang X, and Nielsen D

Subjects
Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, RNA, Bacterial genetics, Escherichia coli drug effects, Escherichia coli genetics, Escherichia coli metabolism, Styrene toxicity, Transcription, Genetic
Abstract

The global transcriptional response of Escherichia coli to styrene and potential influence of exposure source was determined by performing RNA sequencing (RNA-seq) analysis on both styrene-producing and styrene-exposed cells. In both cases, styrene exposure appears to cause both cell envelope and DNA damage, to which cells respond by down-regulating key genes/pathways involved in DNA replication, protein production, and cell wall biogenesis. Among the most significantly up-regulated genes were those involved with phage shock protein response (e.g. pspABCDE/G), general stress regulators (e.g. marA, rpoH), and membrane-altering genes (notably, bhsA, ompR, ldtC), whereas efflux transporters were, surprisingly, unaffected. Subsequent studies with styrene addition demonstrate how strains lacking ompR [involved in controlling outer membrane (OM) composition/osmoregulation] or any of tolQ, tolA, or tolR (involved in OM constriction) each displayed over 40% reduced growth relative to wild-type. Conversely, despite reducing basal fitness, overexpression of plsX (involved in phospholipid biosynthesis) led to 70% greater growth when styrene exposed. These collective differences point to the likely importance of OM properties in controlling native styrene tolerance. Overall, the collective behaviours suggest that, regardless of source, prolonged exposure to inhibitory styrene levels causes cells to shift from'growth mode' to 'survival mode', redistributing cellular resources to fuel native tolerance mechanisms., (© The Author(s) 2021. Published by Oxford University Press on behalf of Society of Industrial Microbiology and Biotechnology.)

Published
2021
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11. CRISPAltRations: a validated cloud-based approach for interrogation of double-strand break repair mediated by CRISPR genome editing.

Author

Kurgan G, Turk R, Li H, Roberts N, Rettig GR, Jacobi AM, Tso L, Sturgeon M, Mertens M, Noten R, Florus K, Behlke MA, Wang Y, and McNeill MS

Abstract

CRISPR systems enable targeted genome editing in a wide variety of organisms by introducing single- or double-strand DNA breaks, which are repaired using endogenous molecular pathways. Characterization of on- and off-target editing events from CRISPR proteins can be evaluated using targeted genome resequencing. We characterized DNA repair fingerprints that result from non-homologous end joining (NHEJ) after double-stranded breaks (DSBs) were introduced by Cas9 or Cas12a for >500 paired treatment/control experiments. We found that building biological understanding of the repair into a novel analysis tool (CRISPAltRations) improved the quality of the results. We validated our software using simulated, targeted amplicon sequencing data (11 guide RNAs [gRNAs] and 603 on- and off-target locations) and demonstrated that CRISPAltRations outperforms other publicly available software tools in accurately annotating CRISPR-associated indels and homology-directed repair (HDR) events. We enable non-bioinformaticians to use CRISPAltRations by developing a web-accessible, cloud-hosted deployment, which allows rapid batch processing of samples in a graphical user interface (GUI) and complies with HIPAA security standards. By ensuring that our software is thoroughly tested, version controlled, and supported with a user interface (UI), we enable resequencing analysis of CRISPR genome editing experiments to researchers no matter their skill in bioinformatics., Competing Interests: G.K., A.M.J., M.S.M., R.T., G.R.R., N.R., H.L., L.T., M.S., Y.W., and M.A.B. are employees or paid contractors/consultants of Integrated DNA Technologies (IDT), which sells reagents used or similar to those used in this manuscript. M.M., K.F., and R.N. are employees of Illumina Inc., which provides a productized cloud-computing platform for doing NGS analysis., (© 2021 Integrated DNA Technologies, Inc.)

Published
2021
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12. Gene replacement of α-globin with β-globin restores hemoglobin balance in β-thalassemia-derived hematopoietic stem and progenitor cells.

Author

Cromer MK, Camarena J, Martin RM, Lesch BJ, Vakulskas CA, Bode NM, Kurgan G, Collingwood MA, Rettig GR, Behlke MA, Lemgart VT, Zhang Y, Goyal A, Zhao F, Ponce E, Srifa W, Bak RO, Uchida N, Majeti R, Sheehan VA, Tisdale JF, Dever DP, and Porteus MH

Subjects
Anemia, Sickle Cell pathology, Animals, Antigens, CD34 metabolism, Dependovirus genetics, Erythrocytes metabolism, Gene Editing, Genes, Reporter, Genetic Loci, Hematopoietic Stem Cell Transplantation, Humans, Mice, Promoter Regions, Genetic genetics, Genetic Therapy, Hematopoietic Stem Cells metabolism, Hemoglobins metabolism, alpha-Globins genetics, beta-Globins genetics, beta-Thalassemia genetics, beta-Thalassemia therapy
Abstract

β-Thalassemia pathology is due not only to loss of β-globin (HBB), but also to erythrotoxic accumulation and aggregation of the β-globin-binding partner, α-globin (HBA1/2). Here we describe a Cas9/AAV6-mediated genome editing strategy that can replace the entire HBA1 gene with a full-length HBB transgene in β-thalassemia-derived hematopoietic stem and progenitor cells (HSPCs), which is sufficient to normalize β-globin:α-globin messenger RNA and protein ratios and restore functional adult hemoglobin tetramers in patient-derived red blood cells. Edited HSPCs were capable of long-term and bilineage hematopoietic reconstitution in mice, establishing proof of concept for replacement of HBA1 with HBB as a novel therapeutic strategy for curing β-thalassemia.

Published
2021
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13. Targeting a cytokine checkpoint enhances the fitness of armored cord blood CAR-NK cells.

Author

Daher M, Basar R, Gokdemir E, Baran N, Uprety N, Nunez Cortes AK, Mendt M, Kerbauy LN, Banerjee PP, Shanley M, Imahashi N, Li L, Lim FLWI, Fathi M, Rezvan A, Mohanty V, Shen Y, Shaim H, Lu J, Ozcan G, Ensley E, Kaplan M, Nandivada V, Bdiwi M, Acharya S, Xi Y, Wan X, Mak D, Liu E, Jiang XR, Ang S, Muniz-Feliciano L, Li Y, Wang J, Kordasti S, Petrov N, Varadarajan N, Marin D, Brunetti L, Skinner RJ, Lyu S, Silva L, Turk R, Schubert MS, Rettig GR, McNeill MS, Kurgan G, Behlke MA, Li H, Fowlkes NW, Chen K, Konopleva M, Champlin RE, Shpall EJ, and Rezvani K

Subjects
Aerobiosis, Animals, Antigens, CD19 immunology, Burkitt Lymphoma pathology, Burkitt Lymphoma therapy, CRISPR-Cas Systems, Cell Line, Tumor, Gene Knockout Techniques, Glycolysis, Humans, Immune Checkpoint Inhibitors pharmacology, Interleukin-15 metabolism, Killer Cells, Natural immunology, Killer Cells, Natural metabolism, Killer Cells, Natural transplantation, Mechanistic Target of Rapamycin Complex 1 physiology, Mice, Neoplasm Proteins genetics, Neoplasm Proteins physiology, Proto-Oncogene Proteins c-akt physiology, Receptors, Chimeric Antigen, Signal Transduction physiology, Suppressor of Cytokine Signaling Proteins genetics, Suppressor of Cytokine Signaling Proteins physiology, Xenograft Model Antitumor Assays, Fetal Blood cytology, Immunotherapy, Adoptive, Interleukin-15 genetics, Killer Cells, Natural drug effects, Neoplasm Proteins antagonists & inhibitors, Suppressor of Cytokine Signaling Proteins antagonists & inhibitors
Abstract

Immune checkpoint therapy has resulted in remarkable improvements in the outcome for certain cancers. To broaden the clinical impact of checkpoint targeting, we devised a strategy that couples targeting of the cytokine-inducible Src homology 2-containing (CIS) protein, a key negative regulator of interleukin 15 (IL-15) signaling, with fourth-generation "armored" chimeric antigen receptor (CAR) engineering of cord blood-derived natural killer (NK) cells. This combined strategy boosted NK cell effector function through enhancing the Akt/mTORC1 axis and c-MYC signaling, resulting in increased aerobic glycolysis. When tested in a lymphoma mouse model, this combined approach improved NK cell antitumor activity more than either alteration alone, eradicating lymphoma xenografts without signs of any measurable toxicity. We conclude that targeting a cytokine checkpoint further enhances the antitumor activity of IL-15-secreting armored CAR-NK cells by promoting their metabolic fitness and antitumor activity. This combined approach represents a promising milestone in the development of the next generation of NK cells for cancer immunotherapy., (© 2021 by The American Society of Hematology.)

Published
2021
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14. Large-scale GMP-compliant CRISPR-Cas9-mediated deletion of the glucocorticoid receptor in multivirus-specific T cells.

Author

Basar R, Daher M, Uprety N, Gokdemir E, Alsuliman A, Ensley E, Ozcan G, Mendt M, Hernandez Sanabria M, Kerbauy LN, Nunez Cortes AK, Li L, Banerjee PP, Muniz-Feliciano L, Acharya S, Fowlkes NW, Lu J, Li S, Mielke S, Kaplan M, Nandivada V, Bdaiwi M, Kontoyiannis AD, Li Y, Liu E, Ang S, Marin D, Brunetti L, Gundry MC, Turk R, Schubert MS, Rettig GR, McNeill MS, Kurgan G, Behlke MA, Champlin R, Shpall EJ, and Rezvani K

Subjects
Gene Editing, Humans, Receptors, Glucocorticoid genetics, T-Lymphocytes, CRISPR-Cas Systems, Clustered Regularly Interspaced Short Palindromic Repeats
Abstract

Virus-specific T cells have proven highly effective for the treatment of severe and drug-refractory infections after hematopoietic stem cell transplant (HSCT). However, the efficacy of these cells is hindered by the use of glucocorticoids, often given to patients for the management of complications such as graft-versus-host disease. To address this limitation, we have developed a novel strategy for the rapid generation of good manufacturing practice (GMP)-grade glucocorticoid-resistant multivirus-specific T cells (VSTs) using clustered regularly interspaced short palindromic repeats (CRISPR)-CRISPR-associated protein 9 (Cas9) gene-editing technology. We have shown that deleting the nuclear receptor subfamily 3 group C member 1 (NR3C1; the gene encoding for the glucocorticoid receptor) renders VSTs resistant to the lymphocytotoxic effect of glucocorticoids. NR3C1-knockout (KO) VSTs kill their targets and proliferate successfully in the presence of high doses of dexamethasone both in vitro and in vivo. Moreover, we developed a protocol for the rapid generation of GMP-grade NR3C1 KO VSTs with high on-target activity and minimal off-target editing. These genetically engineered VSTs promise to be a novel approach for the treatment of patients with life-threatening viral infections post-HSCT on glucocorticoid therapy., (© 2020 by The American Society of Hematology.)

Published
2020
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15. Engineering transport systems for microbial production.

Author

Onyeabor M, Martinez R, Kurgan G, and Wang X

Subjects
Bacteria genetics, Biological Transport, Industrial Microbiology, Bacteria metabolism, Genetic Engineering, Membrane Transport Proteins, Metabolic Engineering, Metabolic Networks and Pathways genetics
Abstract

The rapid development in the field of metabolic engineering has enabled complex modifications of metabolic pathways to generate a diverse product portfolio. Manipulating substrate uptake and product export is an important research area in metabolic engineering. Optimization of transport systems has the potential to enhance microbial production of renewable fuels and chemicals. This chapter comprehensively reviews the transport systems critical for microbial production as well as current genetic engineering strategies to improve transport functions and thus production metrics. In addition, this chapter highlights recent advancements in engineering microbial efflux systems to enhance cellular tolerance to industrially relevant chemical stress. Lastly, future directions to address current technological gaps are discussed., (© 2020 Elsevier Inc. All rights reserved.)

Published
2020
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16. Identification of major malate export systems in an engineered malate-producing Escherichia coli aided by substrate similarity search.

Author

Kurgan G, Kurgan L, Schneider A, Onyeabor M, Rodriguez-Sanchez Y, Taylor E, Martinez R, Carbonell P, Shi X, Gu H, and Wang X

Subjects
Bacterial Proteins genetics, Citric Acid metabolism, Dicarboxylic Acid Transporters genetics, Escherichia coli Proteins genetics, Fermentation genetics, Genetic Engineering, Organic Anion Transporters genetics, Succinic Acid metabolism, Tartrates metabolism, Biological Transport genetics, Carrier Proteins genetics, Escherichia coli genetics, Escherichia coli metabolism, Malates metabolism
Abstract

Optimization of export mechanisms for valuable extracellular products is important for the development of efficient microbial production processes. Identification of the relevant export mechanism is the prerequisite step for product export optimization. In this work, we identified transporters involved in malate export in an engineered L-malate-producing Escherichia coli strain using cheminformatics-guided genetics tests. Among all short-chain di- or tricarboxylates with known transporters in E. coli, citrate, tartrate, and succinate are most chemically similar to malate as estimated by their molecular signatures. Inactivation of three previously reported transporters for succinate, tartrate, and citrate, DcuA, TtdT, and CitT, respectively, dramatically decreased malate production and fermentative growth, suggesting that these transporters have substrate promiscuity for different short-chain organic acids and constitute the major malate export system in E. coli. Malate export deficiency led to an increase in cell sizes and accumulation of intracellular metabolites related to malate metabolism.

Published
2019
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17. Parallel experimental evolution reveals a novel repressive control of GalP on xylose fermentation in Escherichia coli.

Author

Kurgan G, Sievert C, Flores A, Schneider A, Billings T, Panyon L, Morris C, Taylor E, Kurgan L, Cartwright R, and Wang X

Subjects
Catabolite Repression, Escherichia coli genetics, Escherichia coli Proteins genetics, Fermentation, Metabolic Engineering, Monosaccharide Transport Proteins genetics, Mutation, Succinic Acid metabolism, Xylose genetics, Escherichia coli metabolism, Escherichia coli Proteins metabolism, Monosaccharide Transport Proteins metabolism, Xylose metabolism
Abstract

Efficient xylose utilization will facilitate microbial conversion of lignocellulosic sugar mixtures into valuable products. In Escherichia coli, xylose catabolism is controlled by carbon catabolite repression (CCR). However, in E. coli such as the succinate-producing strain KJ122 with disrupted CCR, xylose utilization is still inhibited under fermentative conditions. To probe the underlying genetic mechanisms inhibiting xylose utilization, we evolved KJ122 to enhance its xylose fermentation abilities in parallel and characterized the potential convergent genetic changes shared by multiple independently evolved strains. Whole-genome sequencing revealed that convergent mutations occurred in the galactose regulon during adaptive laboratory evolution potentially decreasing the transcriptional level or the activity of GalP, a galactose permease. We showed that deletion of galP increased xylose utilization in both KJ122 and wild-type E. coli, demonstrating a common repressive role of GalP for xylose fermentation. Concomitantly, induced expression of galP from a plasmid repressed xylose fermentation. Transcriptome analysis using RNA sequencing indicates that galP inactivation increases transcription levels of many catabolic genes for secondary sugars including xylose and arabinose. The repressive role of GalP for fermenting secondary sugars in E. coli suggests that utilization of GalP as a substitute glucose transporter is undesirable for conversion of lignocellulosic sugar mixtures., (© 2019 Wiley Periodicals, Inc.)

Published
2019
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18. Bioprospecting of Native Efflux Pumps To Enhance Furfural Tolerance in Ethanologenic Escherichia coli .

Author

Kurgan G, Panyon LA, Rodriguez-Sanchez Y, Pacheco E, Nieves LM, Mann R, Nielsen DR, and Wang X

Subjects
Bioprospecting, Escherichia coli Proteins genetics, Fermentation, Furaldehyde analogs & derivatives, Genetic Engineering, Lignin metabolism, Multidrug Resistance-Associated Proteins genetics, Escherichia coli genetics, Escherichia coli metabolism, Escherichia coli Proteins metabolism, Ethanol metabolism, Furaldehyde metabolism, Multidrug Resistance-Associated Proteins metabolism
Abstract

Efficient microbial conversion of lignocellulose into valuable products is often hindered by the presence of furfural, a dehydration product of pentoses in hemicellulose sugar syrups derived from woody biomass. For a cost-effective lignocellulose microbial conversion, robust biocatalysts are needed that can tolerate toxic inhibitors while maintaining optimal metabolic activities. A comprehensive plasmid-based library encoding native multidrug resistance (MDR) efflux pumps, porins, and select exporters from Escherichia coli was screened for furfural tolerance in an ethanologenic E. coli strain. Small multidrug resistance (SMR) pumps, such as SugE and MdtJI, as well as a lactate/glycolate:H + symporter, LldP, conferred furfural tolerance in liquid culture tests. Expression of the SMR pump potentially increased furfural efflux and cellular viability upon furfural assault, suggesting novel activities for SMR pumps as furfural efflux proteins. Furthermore, induced expression of mdtJI enhanced ethanol fermentative production of LY180 in the presence of furfural or 5-hydroxymethylfurfural, further demonstrating the applications of SMR pumps. This work describes an effective approach to identify useful efflux systems with desired activities for nonnative toxic chemicals and provides a platform to further enhance furfural efflux by protein engineering and mutagenesis. IMPORTANCE Lignocellulosic biomass, especially agricultural residues, represents an important potential feedstock for microbial production of renewable fuels and chemicals. During the deconstruction of hemicellulose by thermochemical processes, side products that inhibit cell growth and production, such as furan aldehydes, are generated, limiting cost-effective lignocellulose conversion. Here, we developed a new approach to increase cellular tolerance by expressing multidrug resistance (MDR) pumps with putative efflux activities for furan aldehydes. The developed plasmid library and screening methods may facilitate new discoveries of MDR pumps for diverse toxic chemicals important for microbial conversion., (Copyright © 2019 American Society for Microbiology.)

Published
2019
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