Chemical Isotope Labeling LC-MS for Monitoring Disease Progression and Treatment in Animal Models: Plasma Metabolomics Study of Osteoarthritis Rat Model

Chen, Deying; Su, Xiaoling; Wang, Nan; Li, Yunong; Yin, Hua; Liang, Li; Li, Lanjuan

doi:10.1038/srep40543

Cited by 21 publications

(10 citation statements)

References 69 publications

(73 reference statements)

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“…The rat model used for metabolomics study of rheumatoid arthritis (RA) has been described previously. 18 The samples collected from the rats consisted of 7 groups, including a group of normal controls (n = 96), RA, and other treated rats. In total, there were 468 samples, which were processed and analyzed in three batches.…”

Section: Plasma Samples and Sample Processingmentioning

confidence: 99%

“…Each sample was labeled using 12 C-dansylation after protein precipitation, and the resultant labeled sample was analyzed by LC-UV to measure the total concentration of labeled metabolites for sample amount normalization. 18,19 Based on the total concentration, an appropriate volume of an individual unlabeled sample was taken to mix with an equal mole amount of other unlabeled samples to generate a pooled sample, which was then labeled by 13 C-dansylation. An equal mole amount of the 12 C-labeled individual sample and the 13 Clabeled pooled sample was mixed for LC-TOF-MS analysis.…”

Section: Plasma Samples and Sample Processingmentioning

confidence: 99%

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High tolerance to instrument drifts by differential chemical isotope labeling LC‐MS: A case study of the effect of LC leak in long‐term sample runs on quantitative metabolome analysis

et al. 2020

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Metabolomics study of a biological system often involves the analysis of many comparative samples over a period of several days or weeks. This process of long-term sample runs can encounter unexpected instrument drifts such as small leaks in liquid chromatography-mass spectrometry (LC-MS), degradation of column performance, and MS signal intensity change. A robust analytical method should ideally tolerate these instrumental drifts as much as possible. In this work, we report a case study to demonstrate the high tolerance of differential chemical isotope labeling (CIL) LC-MS method for quantitative metabolome analysis. In a study of using a rat model to examine the metabolome changes during rheumatoid arthritis (RA) disease development and treatment, over 468 samples were analyzed over a period of 15 days in three batches. During the sample runs, a small leak in LC was discovered after a batch of analyses was completed. Reanalysis of these samples was not an option as sample amounts were limited. To overcome the problem caused by the small leak, we applied a method of retention time correction to the LC-MS data to align peak pairs from different runs with different degrees of leak, followed by peak ratio calculation and analysis. Herein, we illustrate that using 12 C-/ 13 C-peak pair intensity values in CIL LC-MS as a measurement of concentration changes in different samples could tolerate the signal drifts, while using the absolute intensity values (ie, 12 C-peak as in conventional LC-MS) was not as reliable. We hope that the case study illustrated and the method of overcoming the small-leak-caused signal drifts can be helpful to others who may encounter this kind of situation in long-term sample runs.

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Section: Plasma Samples and Sample Processingmentioning

confidence: 99%

Section: Plasma Samples and Sample Processingmentioning

confidence: 99%

High tolerance to instrument drifts by differential chemical isotope labeling LC‐MS: A case study of the effect of LC leak in long‐term sample runs on quantitative metabolome analysis

et al. 2020

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“…Well-controlled animal models offer inherent phenotypes for specific diseases or abnormal conditions. Therefore, biological samples from animal models are often used in metabolomics studies [86,87,88]. However, only a few metabolomics studies have been conducted using animal hair.…”

Section: Use In Animal Studiesmentioning

confidence: 99%

Hair Metabolomics in Animal Studies and Clinical Settings

et al. 2019

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Metabolomics is a powerful tool used to understand comprehensive changes in the metabolic response and to study the phenotype of an organism by instrumental analysis. It most commonly involves mass spectrometry followed by data mining and metabolite assignment. For the last few decades, hair has been used as a valuable analytical sample to investigate retrospective xenobiotic exposure as it provides a wider window of detection than other biological samples such as saliva, plasma, and urine. Hair contains functional metabolomes such as amino acids and lipids. Moreover, segmental analysis of hair based on its growth rate can provide information on metabolic changes over time. Therefore, it has great potential as a metabolomics sample to monitor chronic diseases, including drug addiction or abnormal conditions. In the current review, the latest applications of hair metabolomics in animal studies and clinical settings are highlighted. For this purpose, we review and discuss the characteristics of hair as a metabolomics sample, the analytical techniques employed in hair metabolomics and the consequence of hair metabolome alterations in recent studies. Through this, the value of hair as an alternative biological sample in metabolomics is highlighted.

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“…In rat models of OA, changes to amino acid metabolism are also observed in urine [41]. Again in rats, a longitudinal metabolomic analysis of plasma showed that there are significant and time-dependent changes in products of lysine metabolism after surgical induction of OA [42]. This further suggests that amino acid metabolism may contribute to OA pathology or that select amino acid levels could be used as biomarkers of OA incidence and progression.…”

Section: The Local and Systemic Metabolomes Of Osteoarthritismentioning

confidence: 99%

The Metabolome and Osteoarthritis: Possible Contributions to Symptoms and Pathology

Rockel

Kapoor

2018

Metabolites

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Osteoarthritis (OA) is a progressive, deteriorative disease of articular joints. Although traditionally viewed as a local pathology, biomarker exploration has shown that systemic changes can be observed. These include changes to cytokines, microRNAs, and more recently, metabolites. The metabolome is the set of metabolites within a biological sample and includes circulating amino acids, lipids, and sugar moieties. Recent studies suggest that metabolites in the synovial fluid and blood could be used as biomarkers for OA incidence, prognosis, and response to therapy. However, based on clinical, demographic, and anthropometric factors, the local synovial joint and circulating metabolomes may be patient specific, with select subsets of metabolites contributing to OA disease. This review explores the contribution of the local and systemic metabolite changes to OA, and their potential impact on OA symptoms and disease pathogenesis.

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Chemical Isotope Labeling LC-MS for Monitoring Disease Progression and Treatment in Animal Models: Plasma Metabolomics Study of Osteoarthritis Rat Model

Cited by 21 publications

References 69 publications

High tolerance to instrument drifts by differential chemical isotope labeling LC‐MS: A case study of the effect of LC leak in long‐term sample runs on quantitative metabolome analysis

High tolerance to instrument drifts by differential chemical isotope labeling LC‐MS: A case study of the effect of LC leak in long‐term sample runs on quantitative metabolome analysis

Hair Metabolomics in Animal Studies and Clinical Settings

The Metabolome and Osteoarthritis: Possible Contributions to Symptoms and Pathology

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