Inhibitor

Bibliography

Biblio print

Tree Display

AceDB Schema

XML Display

Feedback

Paper(s) concerning alkyne-PEG-FP

2 reference(s) found.
Listing paper details in reverse chronological order.
We are grateful to Keith Bradnam for improvment of this script

Title: Small-Molecule Probes Reveal Esterases with Persistent Activity in Dormant and Reactivating Mycobacterium tuberculosis
Tallman KR, Levine SR, Beatty KE
Ref: ACS Infect Dis, 2:936, 2016 : PubMed
Abstract


ESTHER: Tallman_2016_ACS.Infect.Dis_2_936
PubMedSearch: Tallman 2016 ACS.Infect.Dis 2 936
PubMedID: 27690385
Gene_locus related to this paper: myctu-rv0183, myctu-Rv1399c, myctu-RV1683, myctu-Rv2284, myctu-Rv2970c, myctu-ym24
Inhibitor(s) related to this paper: alkyne-PEG-FP

Abstract

Mycobacterium tuberculosis (Mtb) is the deadliest bacterial pathogen in the world. An estimated one-third of humans harbor Mtb in a dormant state. These asymptomatic, latent infections impede tuberculosis eradication due to the long-term potential for reactivation. Dormant Mtb has reduced enzymatic activity, but hydrolases that remain active facilitate pathogen survival. We targeted Mtb esterases, a diverse set of enzymes in the serine hydrolase family, and studied their activities using both activity-based probes (ABPs) and fluorogenic esterase substrates. These small-molecule probes revealed functional esterases in active, dormant, and reactivating cultures. Using ABPs, we identified five esterases that remained active in dormant Mtb, including LipM (Rv2284), LipN (Rv2970c), CaeA (Rv2224c), Rv0183, and Rv1683. Three of these, CaeA, Rv0183, and Rv1683, were catalytically active in all three culture conditions. Fluorogenic probes additionally revealed LipH (Rv1399c), Culp1 (Rv1984c), and Rv3036c esterase activity in dormant and active cultures. Esterases with persistent activity are potential diagnostic biomarkers or therapeutic targets for Mtb-infected individuals with latent or active tuberculosis.



        

Title: Multiplexed activity-based protein profiling of the human pathogen Aspergillus fumigatus reveals large functional changes upon exposure to human serum
Wiedner SD, Burnum KE, Pederson LM, Anderson LN, Fortuin S, Chauvigne-Hines LM, Shukla AK, Ansong C, Panisko EA and Wright AT <1 more author(s)> Wiedner SD, Burnum KE, Pederson LM, Anderson LN, Fortuin S, Chauvigne-Hines LM, Shukla AK, Ansong C, Panisko EA, Smith RD, Wright AT (- 1)
Ref: Journal of Biological Chemistry, 287:33447, 2012 : PubMed
Abstract


ESTHER: Wiedner_2012_J.Biol.Chem_287_33447
PubMedSearch: Wiedner 2012 J.Biol.Chem 287 33447
PubMedID: 22865858
Inhibitor(s) related to this paper: alkyne-PEG-FP

Abstract

Environmental adaptability is critical for survival of the fungal human pathogen Aspergillus fumigatus in the immunocompromised host lung. We hypothesized that exposure of the fungal pathogen to human serum would lead to significant alterations to the organism's physiology, including metabolic activity and stress response. Shifts in functional pathway and corresponding enzyme reactivity of A. fumigatus upon exposure to the human host may represent much needed prognostic indicators of fungal infection. To address this, we employed a multiplexed activity-based protein profiling (ABPP) approach coupled to quantitative mass spectrometry-based proteomics to measure broad enzyme reactivity of the fungus cultured with and without human serum. ABPP showed a shift from aerobic respiration to ethanol fermentation and utilization over time in the presence of human serum, which was not observed in serum-free culture. Our approach provides direct insight into this pathogen's ability to survive, adapt, and proliferate. Additionally, our multiplexed ABPP approach captured a broad swath of enzyme reactivity and functional pathways and provides a method for rapid assessment of the A. fumigatus response to external stimuli.