A covalent reporter of β-lactamase activity for fluorescent imaging and rapid screening of antibiotic-resistant bacteria

A covalent reporter of β-lactamase activity for fluorescent imaging and rapid screening of antibiotic-resistant bacteria

Bacterial resistance to antibiotics poses a great clinical challenge in fighting serious infectious diseases due to complicated resistant mechanisms and time-consuming testing methods. Chemical reaction-directed covalent labeling of resistance-associated bacterial proteins in the context of a compli...

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Main Authors: Shao, Qing, Zheng, Yan, Dong, Xueming, Tang, Kai, Yan, Xiaomei, Xing, Bengang
Other Authors: School of Physical and Mathematical Sciences
Format: Article
Language:English
Published: 2013
Online Access:https://hdl.handle.net/10356/106609
http://hdl.handle.net/10220/16649
http://dx.doi.org/10.1002/chem.201301654
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Institution: Nanyang Technological University
Language: English
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spelling sg-ntu-dr.10356-1066092019-12-06T22:14:54Z A covalent reporter of β-lactamase activity for fluorescent imaging and rapid screening of antibiotic-resistant bacteria Shao, Qing Zheng, Yan Dong, Xueming Tang, Kai Yan, Xiaomei Xing, Bengang School of Physical and Mathematical Sciences Bacterial resistance to antibiotics poses a great clinical challenge in fighting serious infectious diseases due to complicated resistant mechanisms and time-consuming testing methods. Chemical reaction-directed covalent labeling of resistance-associated bacterial proteins in the context of a complicated environment offers great opportunity for the in-depth understanding of the biological basis conferring drug resistance, and for the development of effective diagnostic approaches. In the present study, three fluorogenic reagents LRBL1–3 for resistant bacteria labeling have been designed and prepared on the basis of fluorescence resonance energy transfer (FRET). The hydrolyzed probes could act as reactive electrophiles to attach the enzyme, β-lactamase, and thus facilitated the covalent labeling of drug resistant bacterial strains. SDS electrophoresis and MALDI-TOF mass spectrometry characterization confirmed that these probes were sensitive and specific to β-lactamase and could therefore serve for covalent and localized fluorescence labeling of the enzyme structure. Moreover, this β-lactamase-induced covalent labeling provides quantitative analysis of the resistant bacterial population (down to 5 %) by high resolution flow cytometry, and allows single-cell detection and direct observation of bacterial enzyme activity in resistant pathogenic species. This approach offers great promise for clinical investigations and microbiological research. 2013-10-21T04:00:03Z 2019-12-06T22:14:54Z 2013-10-21T04:00:03Z 2019-12-06T22:14:54Z 2013 2013 Journal Article Shao, Q., Zheng, Y., Dong, X., Tang, K., Yan, X.,& Xing, B. (2013). A Covalent Reporter of β-Lactamase Activity for Fluorescent Imaging and Rapid Screening of Antibiotic-Resistant Bacteria. Chemistry - A European Journal, 19(33), 10903-10910. 0947-6539 https://hdl.handle.net/10356/106609 http://hdl.handle.net/10220/16649 http://dx.doi.org/10.1002/chem.201301654 en Chemistry - a European journal
institution Nanyang Technological University
building NTU Library
country Singapore
collection DR-NTU
language English
description Bacterial resistance to antibiotics poses a great clinical challenge in fighting serious infectious diseases due to complicated resistant mechanisms and time-consuming testing methods. Chemical reaction-directed covalent labeling of resistance-associated bacterial proteins in the context of a complicated environment offers great opportunity for the in-depth understanding of the biological basis conferring drug resistance, and for the development of effective diagnostic approaches. In the present study, three fluorogenic reagents LRBL1–3 for resistant bacteria labeling have been designed and prepared on the basis of fluorescence resonance energy transfer (FRET). The hydrolyzed probes could act as reactive electrophiles to attach the enzyme, β-lactamase, and thus facilitated the covalent labeling of drug resistant bacterial strains. SDS electrophoresis and MALDI-TOF mass spectrometry characterization confirmed that these probes were sensitive and specific to β-lactamase and could therefore serve for covalent and localized fluorescence labeling of the enzyme structure. Moreover, this β-lactamase-induced covalent labeling provides quantitative analysis of the resistant bacterial population (down to 5 %) by high resolution flow cytometry, and allows single-cell detection and direct observation of bacterial enzyme activity in resistant pathogenic species. This approach offers great promise for clinical investigations and microbiological research.
author2 School of Physical and Mathematical Sciences
author_facet School of Physical and Mathematical Sciences
Shao, Qing
Zheng, Yan
Dong, Xueming
Tang, Kai
Yan, Xiaomei
Xing, Bengang
format Article
author Shao, Qing
Zheng, Yan
Dong, Xueming
Tang, Kai
Yan, Xiaomei
Xing, Bengang
spellingShingle Shao, Qing
Zheng, Yan
Dong, Xueming
Tang, Kai
Yan, Xiaomei
Xing, Bengang
A covalent reporter of β-lactamase activity for fluorescent imaging and rapid screening of antibiotic-resistant bacteria
author_sort Shao, Qing
title A covalent reporter of β-lactamase activity for fluorescent imaging and rapid screening of antibiotic-resistant bacteria
title_short A covalent reporter of β-lactamase activity for fluorescent imaging and rapid screening of antibiotic-resistant bacteria
title_full A covalent reporter of β-lactamase activity for fluorescent imaging and rapid screening of antibiotic-resistant bacteria
title_fullStr A covalent reporter of β-lactamase activity for fluorescent imaging and rapid screening of antibiotic-resistant bacteria
title_full_unstemmed A covalent reporter of β-lactamase activity for fluorescent imaging and rapid screening of antibiotic-resistant bacteria
title_sort covalent reporter of β-lactamase activity for fluorescent imaging and rapid screening of antibiotic-resistant bacteria
publishDate 2013
url https://hdl.handle.net/10356/106609
http://hdl.handle.net/10220/16649
http://dx.doi.org/10.1002/chem.201301654
_version_ 1681038951669825536

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