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  • Urine metabolic fingerprinting using LC-MS and GC-MS reveals metabolite changes in prostate cancer: A pilot study.

Urine metabolic fingerprinting using LC-MS and GC-MS reveals metabolite changes in prostate cancer: A pilot study.

Journal of pharmaceutical and biomedical analysis (2015-02-17)
Wiktoria Struck-Lewicka, Marta Kordalewska, Renata Bujak, Arlette Yumba Mpanga, Marcin Markuszewski, Julia Jacyna, Marcin Matuszewski, Roman Kaliszan, Michał J Markuszewski
要旨

Prostate cancer (CaP) is a leading cause of cancer deaths in men worldwide. The alarming statistics, the currently applied biomarkers are still not enough specific and selective. In addition, pathogenesis of CaP development is not totally understood. Therefore, in the present work, metabolomics study related to urinary metabolic fingerprinting analyses has been performed in order to scrutinize potential biomarkers that could help in explaining the pathomechanism of the disease and be potentially useful in its diagnosis and prognosis. Urine samples from CaP patients and healthy volunteers were analyzed with the use of high performance liquid chromatography coupled with time of flight mass spectrometry detection (HPLC-TOF/MS) in positive and negative polarity as well as gas chromatography hyphenated with triple quadruple mass spectrometry detection (GC-QqQ/MS) in a scan mode. The obtained data sets were statistically analyzed using univariate and multivariate statistical analyses. The Principal Component Analysis (PCA) was used to check systems' stability and possible outliers, whereas Partial Least Squares Discriminant Analysis (PLS-DA) was performed for evaluation of quality of the model as well as its predictive ability using statistically significant metabolites. The subsequent identification of selected metabolites using NIST library and commonly available databases allows for creation of a list of putative biomarkers and related biochemical pathways they are involved in. The selected pathways, like urea and tricarboxylic acid cycle, amino acid and purine metabolism, can play crucial role in pathogenesis of prostate cancer disease.

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メタノール, anhydrous, 99.8%
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ピリジン, anhydrous, 99.8%
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クロロトリメチルシラン, ≥98.0% (GC)
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N,O-ビス(トリメチルシリル)トリフルオロセトアミド および トリメチルクロロシラン, with 1% trimethylchlorosilane, derivatization grade (GC derivatization), LiChropur
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ヘキサン, anhydrous, 95%
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N,O-ビス(トリメチルシリル)トリフルオロアセトアミド, ≥99%
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クロロトリメチルシラン, purified by redistillation, ≥99%
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メタノール, JIS special grade, ≥99.8%
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ヘプタン, anhydrous, 99%
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メタノール, SAJ first grade, ≥99.5%
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ピリジン, ≥99%
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ペンタデカン酸, 99%
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ペンタデカン酸, ~99% (capillary GC)
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ヘキサン, JIS special grade, ≥96.0%
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メタノール, SAJ special grade
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ヘキサン, HPLC Plus, for HPLC, GC, and residue analysis, ≥95%
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メタノール, suitable for HPLC
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クロロトリメチルシラン, Wacker Chemie AG, ≥99.0% (GC)
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メタノール, HPLC Plus, ≥99.9%, poly-coated bottles
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ヘキサン, suitable for HPLC
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ヘキサン, SAJ first grade, ≥95.0%
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メタノール, suitable for NMR (reference standard)
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クロロトリメチルシラン 溶液, 1.0 M in THF
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ヘキサン, JIS 300, ≥96.0%, suitable for residue analysis
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ヘプタン, JIS special grade, ≥99.0%
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メタノール, JIS 300, ≥99.8%, suitable for residue analysis
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