Suite of Activity-Based Probes for Cellulose-Degrading Enzymes

Chauvigné-Hines, Lacie M.; Anderson, Lindsey; Weaver, Holly M.; Brown, Joseph N.; Koech, Phillip K.; Nicora, Carrie; Hofstad, Beth A.; Smith, Richard D.; Wilkins, Michael J.; Callister, Stephen; Wright, Aaron

doi:10.1021/ja309790w

Cited by 69 publications

(68 citation statements)

References 61 publications

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“…19 Proteins were digested on-resin with trypsin, and the resulting peptides were collected and analyzed on a LTQ instrument by LC-MS as described previously. 20 Generated MS/MS spectra were searched using the MSGF+ algorithm 21 against the publicly available G. gallus or M. gallopavo translated genome sequences, and rescored using the MS-GF approach. 21 Identified peptides of at least six amino acids in length having MS-GF scores ≤1 × 10 −10 , corresponding to an estimated false discovery rate (FDR) <1% at the peptide level, were used for analysis.…”

Section: Methodsmentioning

confidence: 99%

Role of Cytochrome P450 Hydroxylase in the Decreased Accumulation of Vitamin E in Muscle from Turkeys Compared to that from Chickens

Perez

Richards

Berres

et al. 2016

J. Agric. Food Chem.

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Turkeys and chickens reared to 5 weeks of age and fed diets with feedstuffs low in endogenous tocopherols were examined. Treatments included feed supplemented with RRR (natural source vitamin E) alpha tocopheryl acetate (AcT, 35 mg/kg feed) and all-racemic (synthetic vitamin E) AcT (10 and 58 mg/kg feed). Alpha tocopherol hydroxylase activity was greater in liver microsomes prepared from turkeys compared to that from chickens (p < 0.01). Alpha and gamma tocopherol metabolites were higher in turkey bile than in chicken when assessing the RRR AcT diet and the all-racemic AcT diet at 58 mg/kg feed (p < 0.01). Turkey cytochrome P450 2C29 was increased relative to its chicken ortholog on the basis of RNA-Seq transcript abundance (p < 0.001) and activity-based protein profiling (p < 0.01) of liver tissue. Alpha tocopherol concentrations in plasma, liver, and muscle from turkey were lower than the respective tissues from chicken (p < 0.05). Lipid oxidation was greater in turkey thigh than in chicken (p < 0.05). These results suggest that elevated tocopherol metabolism by cytochrome P450 hydroxylase(s) in turkeys contributes to the decreased accumulation of alpha tocopherol in turkey tissues compared to that of chickens.

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Section: Methodsmentioning

confidence: 99%

Role of Cytochrome P450 Hydroxylase in the Decreased Accumulation of Vitamin E in Muscle from Turkeys Compared to that from Chickens

Perez

Richards

Berres

et al. 2016

J. Agric. Food Chem.

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“…Following probe incubation, biotin was appended by CuAAC, followed by removal of excess CuAAC reagents by concentration and buffer washing using an Amicon Millipore centrifugal device. 27 Samples were normalized to 1 mg protein before enriching on streptavidin agarose resin. Enriched proteins were washed, digested with trypsin, and vialed for subsequent MS analysis as described previously.…”

Section: Methodsmentioning

confidence: 99%

“…Enriched proteins were washed, digested with trypsin, and vialed for subsequent MS analysis as described previously. 27 …”

Section: Methodsmentioning

confidence: 99%

“…26 We recently developed a suite of activity-based probes (ABPs) for glycoside hydrolases, and used them to characterize anaerobic lignocellulose degradation in the bacterium Clostridium thermocellum. 27 Our ABPs are developed as affinity-based inhibitors of glycoside hydrolases (GHs), forming a covalent bond upon reaction with the catalytic domains of target enzymes. Probes are also compatible with copper-mediated azide–alkyne cyclo-additions that permit both fluorescent and LC-MS characterization of ABP-labeled proteins.…”

Section: Introductionmentioning

confidence: 99%

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Activity-based protein profiling of secreted cellulolytic enzyme activity dynamics in Trichoderma reesei QM6a, NG14, and RUT-C30

et al. 2013

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Lignocellulosic biomass has great promise as a highly abundant and renewable source for the production of biofuels. However, the recalcitrant nature of lignocellulose toward hydrolysis into soluble sugars remains a significant challenge to harnessing the potential of this source of bioenergy. A primary method for deconstructing lignocellulose is via chemical treatments, high temperatures, and hydrolytic enzyme cocktails, many of which are derived from the fungus Trichoderma reesei. Herein, we use an activity-based probe for glycoside hydrolases to rapidly identify optimal conditions for maximum enzymatic lignocellulose deconstruction. We also demonstrate that subtle changes to enzyme composition and activity in various strains of T. reesei can be readily characterized by our probe approach. The approach also permits multimodal measurements, including fluorescent gel-based analysis of activity in response to varied conditions and treatments, and mass spectrometry-based quantitative identification of labelled proteins. We demonstrate the promise this probe approach holds to facilitate rapid production of enzyme cocktails for high-efficiency lignocellulose deconstruction to accommodate high-yield biofuel production.

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“…Activitybased probes have been designed to detect a number of bacterial proteins, such as sulfatases 85,86 , serine proteases 87 , the cell wall biosynthetic protein MurA 88 , glycoside hydrolases 89 , redox-sensitive proteins 90,91 and histidine kinases 92 ; however, most of these probes have been used only in gel-based analyses. One additional strategy that has been applied to bacterial imaging is the use of a probe that becomes fluorescent upon turnover by nitroreductase.…”

Section: Additional Small-molecule Probesmentioning

confidence: 99%

Progress and prospects for small-molecule probes of bacterial imaging

Kocaoglu

Carlson

2016

Nat Chem Biol

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Fluorescence microscopy is an essential tool for the exploration of cell growth, division, transcription and translation in eukaryotes and prokaryotes alike. Despite the rapid development of techniques to study bacteria, the size of these organisms (1–10 μm) and their robust and largely impenetrable cell envelope present major challenges in imaging experiments. Fusion-based strategies, such as attachment of the protein of interest to a fluorescent protein or epitope tag, are by far the most common means for examining protein localization and expression in prokaryotes. While valuable, the use of genetically encoded tags can result in mislocalization or altered activity of the desired protein, does not provide a readout of the catalytic state of enzymes and cannot enable visualization of many other important cellular components, such as peptidoglycan, lipids, nucleic acids or glycans. Here, we highlight the use of biomolecule-specific small-molecule probes for imaging in bacteria.

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Suite of Activity-Based Probes for Cellulose-Degrading Enzymes

Cited by 69 publications

References 61 publications

Role of Cytochrome P450 Hydroxylase in the Decreased Accumulation of Vitamin E in Muscle from Turkeys Compared to that from Chickens

Role of Cytochrome P450 Hydroxylase in the Decreased Accumulation of Vitamin E in Muscle from Turkeys Compared to that from Chickens

Activity-based protein profiling of secreted cellulolytic enzyme activity dynamics in Trichoderma reesei QM6a, NG14, and RUT-C30

Progress and prospects for small-molecule probes of bacterial imaging

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