OPTIMIZATION OF DEPROTEINIZATION METHODS, HPLC METHOD DEVELOPMENT AND VALIDATION FOR QUANTIFICATION OF 6Β-HYDROXYTESTOSTERONE IN CELL CULTURE MEDIA

Testosterone is commonly used as a marker probe drug for CYP3A4 metabolic activity. Accurate measurement of its metabolite, 6β-hydroxytestosterone in cell culture media is very crucial. This study aimed to optimize solvent extraction method as well as to develop and validate HPLC analytical method f...

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Published in:Jurnal Teknologi
Main Author: Ridhwan M.J.M.; Mutalib N.A.; Latip N.A.; Rasol N.E.; Bakar S.I.A.; Ismail N.H.
Format: Article
Language:English
Published: Penerbit UTM Press 2024
Online Access:https://www.scopus.com/inward/record.uri?eid=2-s2.0-85180491358&doi=10.11113%2fjurnalteknologi.v86.19861&partnerID=40&md5=6ad31eb7bba9e80a9c36ea1f3f437868
id 2-s2.0-85180491358
spelling 2-s2.0-85180491358
Ridhwan M.J.M.; Mutalib N.A.; Latip N.A.; Rasol N.E.; Bakar S.I.A.; Ismail N.H.
OPTIMIZATION OF DEPROTEINIZATION METHODS, HPLC METHOD DEVELOPMENT AND VALIDATION FOR QUANTIFICATION OF 6Β-HYDROXYTESTOSTERONE IN CELL CULTURE MEDIA
2024
Jurnal Teknologi
86
1
10.11113/jurnalteknologi.v86.19861
https://www.scopus.com/inward/record.uri?eid=2-s2.0-85180491358&doi=10.11113%2fjurnalteknologi.v86.19861&partnerID=40&md5=6ad31eb7bba9e80a9c36ea1f3f437868
Testosterone is commonly used as a marker probe drug for CYP3A4 metabolic activity. Accurate measurement of its metabolite, 6β-hydroxytestosterone in cell culture media is very crucial. This study aimed to optimize solvent extraction method as well as to develop and validate HPLC analytical method for the quantification of 6β-hydroxytestosterone. Testosterone and 6β-hydroxytestost-erone were extracted from culture media using different solvents and were analyzed using BCA assay and HPLC. The separation was performed at 0.7 mL/min flow rate, using gradient elution of water:methanol for 38 minutes at 242 nm. Solvent extraction of cell culture media using methanol showed the highest crude extract recovery, yield recovery of compounds, and percentage recovery of compounds and peak areas. Thus, the methanol extraction method was applied to further validate 6β-hydroxytestosterone HPLC analytical method. The specificity of the metabolite peak was excellent without any interference. The linear range was 0.156-5.000 ppm. The precision and accuracy were within acceptable criteria of <15%. Samples were stable at 4 ºC chiller for up to 5 days, in autosampler for 24 hours, and in-20 ºC freezer for up to one month. The method was successfully developed and validated for the quantification of 6β-hydroxytestosterone in cell culture media. © 2024, Penerbit UTM Press. All rights reserved.
Penerbit UTM Press
1279696
English
Article
All Open Access; Gold Open Access
author Ridhwan M.J.M.; Mutalib N.A.; Latip N.A.; Rasol N.E.; Bakar S.I.A.; Ismail N.H.
spellingShingle Ridhwan M.J.M.; Mutalib N.A.; Latip N.A.; Rasol N.E.; Bakar S.I.A.; Ismail N.H.
OPTIMIZATION OF DEPROTEINIZATION METHODS, HPLC METHOD DEVELOPMENT AND VALIDATION FOR QUANTIFICATION OF 6Β-HYDROXYTESTOSTERONE IN CELL CULTURE MEDIA
author_facet Ridhwan M.J.M.; Mutalib N.A.; Latip N.A.; Rasol N.E.; Bakar S.I.A.; Ismail N.H.
author_sort Ridhwan M.J.M.; Mutalib N.A.; Latip N.A.; Rasol N.E.; Bakar S.I.A.; Ismail N.H.
title OPTIMIZATION OF DEPROTEINIZATION METHODS, HPLC METHOD DEVELOPMENT AND VALIDATION FOR QUANTIFICATION OF 6Β-HYDROXYTESTOSTERONE IN CELL CULTURE MEDIA
title_short OPTIMIZATION OF DEPROTEINIZATION METHODS, HPLC METHOD DEVELOPMENT AND VALIDATION FOR QUANTIFICATION OF 6Β-HYDROXYTESTOSTERONE IN CELL CULTURE MEDIA
title_full OPTIMIZATION OF DEPROTEINIZATION METHODS, HPLC METHOD DEVELOPMENT AND VALIDATION FOR QUANTIFICATION OF 6Β-HYDROXYTESTOSTERONE IN CELL CULTURE MEDIA
title_fullStr OPTIMIZATION OF DEPROTEINIZATION METHODS, HPLC METHOD DEVELOPMENT AND VALIDATION FOR QUANTIFICATION OF 6Β-HYDROXYTESTOSTERONE IN CELL CULTURE MEDIA
title_full_unstemmed OPTIMIZATION OF DEPROTEINIZATION METHODS, HPLC METHOD DEVELOPMENT AND VALIDATION FOR QUANTIFICATION OF 6Β-HYDROXYTESTOSTERONE IN CELL CULTURE MEDIA
title_sort OPTIMIZATION OF DEPROTEINIZATION METHODS, HPLC METHOD DEVELOPMENT AND VALIDATION FOR QUANTIFICATION OF 6Β-HYDROXYTESTOSTERONE IN CELL CULTURE MEDIA
publishDate 2024
container_title Jurnal Teknologi
container_volume 86
container_issue 1
doi_str_mv 10.11113/jurnalteknologi.v86.19861
url https://www.scopus.com/inward/record.uri?eid=2-s2.0-85180491358&doi=10.11113%2fjurnalteknologi.v86.19861&partnerID=40&md5=6ad31eb7bba9e80a9c36ea1f3f437868
description Testosterone is commonly used as a marker probe drug for CYP3A4 metabolic activity. Accurate measurement of its metabolite, 6β-hydroxytestosterone in cell culture media is very crucial. This study aimed to optimize solvent extraction method as well as to develop and validate HPLC analytical method for the quantification of 6β-hydroxytestosterone. Testosterone and 6β-hydroxytestost-erone were extracted from culture media using different solvents and were analyzed using BCA assay and HPLC. The separation was performed at 0.7 mL/min flow rate, using gradient elution of water:methanol for 38 minutes at 242 nm. Solvent extraction of cell culture media using methanol showed the highest crude extract recovery, yield recovery of compounds, and percentage recovery of compounds and peak areas. Thus, the methanol extraction method was applied to further validate 6β-hydroxytestosterone HPLC analytical method. The specificity of the metabolite peak was excellent without any interference. The linear range was 0.156-5.000 ppm. The precision and accuracy were within acceptable criteria of <15%. Samples were stable at 4 ºC chiller for up to 5 days, in autosampler for 24 hours, and in-20 ºC freezer for up to one month. The method was successfully developed and validated for the quantification of 6β-hydroxytestosterone in cell culture media. © 2024, Penerbit UTM Press. All rights reserved.
publisher Penerbit UTM Press
issn 1279696
language English
format Article
accesstype All Open Access; Gold Open Access
record_format scopus
collection Scopus
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