Comparison of activity indexes for recognizing enzyme mutants of higher activity with uricase as model

BACKGROUND: For screening a library of enzyme mutants, an efficient and cost-effective method for reliable assay of enzyme activity and a decision method for safe recognition of mutants of higher activity are needed. The comparison of activity concentrations of mutants in lysates of transformed Esch...

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Autores principales: Feng, Juan, Liu, Hongbo, Yang, Xiaolan, Gao, Ang, Liao, Juan, Feng, Liping, Pu, Jun, Xie, Yanling, Long, Gaobo, Li, Yuanli, Liao, Fei
Formato: Online Artículo Texto
Lenguaje:English
Publicado: BioMed Central 2013
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Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3637054/
https://www.ncbi.nlm.nih.gov/pubmed/23594729
http://dx.doi.org/10.1186/1752-153X-7-69
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author Feng, Juan
Liu, Hongbo
Yang, Xiaolan
Gao, Ang
Liao, Juan
Feng, Liping
Pu, Jun
Xie, Yanling
Long, Gaobo
Li, Yuanli
Liao, Fei
author_facet Feng, Juan
Liu, Hongbo
Yang, Xiaolan
Gao, Ang
Liao, Juan
Feng, Liping
Pu, Jun
Xie, Yanling
Long, Gaobo
Li, Yuanli
Liao, Fei
author_sort Feng, Juan
collection PubMed
description BACKGROUND: For screening a library of enzyme mutants, an efficient and cost-effective method for reliable assay of enzyme activity and a decision method for safe recognition of mutants of higher activity are needed. The comparison of activity concentrations of mutants in lysates of transformed Escherichia coli cells against a threshold is unsafe to recognize mutants of higher activity due to variations of both expression levels of mutant proteins and lysis efficiency of transformed cells. Hence, by a spectrophotometric method after verification to measure uricase activity, specific activity calculated from the level of total proteins in a lysate was tested for recognizing a mutant of higher activity. RESULTS: During uricase reaction, the intermediate 5-hydroxyisourate interferes with the assay of uric acid absorbance, but the measurement of absorbance at 293 nm in alkaline borate buffer was reliable for measuring uricase initial rates within a reasonable range. The level of total proteins in a lysate was determined by the Bradford assay. Polyacrylamide gel electrophoresis analysis supported different relative abundance of uricase mutant proteins in their lysates; activity concentrations of uricase in such lysates positively correlated with levels of total proteins. Receiver-operation-curve analysis of activity concentration or specific activity yielded area-under-the-curve close to 1.00 for recognizing a mutant with > 200% improvement of activity. For a mutant with just about 80% improvement of activity, receiver-operation-curve analysis of specific activity gave area-under-the-curve close to 1.00 while the analysis of activity concentration gave smaller area-under-the-curve. With the mean plus 1.4-fold of the standard deviation of specific activity of a starting material as the threshold, uricase mutants whose activities were improved by more than 80% were recognized with higher sensitivity and specificity. CONCLUSION: Specific activity calculated from the level of total proteins is a favorable index for recognizing an enzyme mutant with small improvement of activity.
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spelling pubmed-36370542013-04-27 Comparison of activity indexes for recognizing enzyme mutants of higher activity with uricase as model Feng, Juan Liu, Hongbo Yang, Xiaolan Gao, Ang Liao, Juan Feng, Liping Pu, Jun Xie, Yanling Long, Gaobo Li, Yuanli Liao, Fei Chem Cent J Research Article BACKGROUND: For screening a library of enzyme mutants, an efficient and cost-effective method for reliable assay of enzyme activity and a decision method for safe recognition of mutants of higher activity are needed. The comparison of activity concentrations of mutants in lysates of transformed Escherichia coli cells against a threshold is unsafe to recognize mutants of higher activity due to variations of both expression levels of mutant proteins and lysis efficiency of transformed cells. Hence, by a spectrophotometric method after verification to measure uricase activity, specific activity calculated from the level of total proteins in a lysate was tested for recognizing a mutant of higher activity. RESULTS: During uricase reaction, the intermediate 5-hydroxyisourate interferes with the assay of uric acid absorbance, but the measurement of absorbance at 293 nm in alkaline borate buffer was reliable for measuring uricase initial rates within a reasonable range. The level of total proteins in a lysate was determined by the Bradford assay. Polyacrylamide gel electrophoresis analysis supported different relative abundance of uricase mutant proteins in their lysates; activity concentrations of uricase in such lysates positively correlated with levels of total proteins. Receiver-operation-curve analysis of activity concentration or specific activity yielded area-under-the-curve close to 1.00 for recognizing a mutant with > 200% improvement of activity. For a mutant with just about 80% improvement of activity, receiver-operation-curve analysis of specific activity gave area-under-the-curve close to 1.00 while the analysis of activity concentration gave smaller area-under-the-curve. With the mean plus 1.4-fold of the standard deviation of specific activity of a starting material as the threshold, uricase mutants whose activities were improved by more than 80% were recognized with higher sensitivity and specificity. CONCLUSION: Specific activity calculated from the level of total proteins is a favorable index for recognizing an enzyme mutant with small improvement of activity. BioMed Central 2013-04-17 /pmc/articles/PMC3637054/ /pubmed/23594729 http://dx.doi.org/10.1186/1752-153X-7-69 Text en Copyright © 2013 Feng et al.; licensee Chemistry Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Research Article
Feng, Juan
Liu, Hongbo
Yang, Xiaolan
Gao, Ang
Liao, Juan
Feng, Liping
Pu, Jun
Xie, Yanling
Long, Gaobo
Li, Yuanli
Liao, Fei
Comparison of activity indexes for recognizing enzyme mutants of higher activity with uricase as model
title Comparison of activity indexes for recognizing enzyme mutants of higher activity with uricase as model
title_full Comparison of activity indexes for recognizing enzyme mutants of higher activity with uricase as model
title_fullStr Comparison of activity indexes for recognizing enzyme mutants of higher activity with uricase as model
title_full_unstemmed Comparison of activity indexes for recognizing enzyme mutants of higher activity with uricase as model
title_short Comparison of activity indexes for recognizing enzyme mutants of higher activity with uricase as model
title_sort comparison of activity indexes for recognizing enzyme mutants of higher activity with uricase as model
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3637054/
https://www.ncbi.nlm.nih.gov/pubmed/23594729
http://dx.doi.org/10.1186/1752-153X-7-69
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