Biomonitoring of Aristolactam-DNA Adducts in Human Tissues Using Ultra-Performance Liquid Chromatography/Ion-Trap Mass Spectrometry

Yun, Byeong Hwa; Rosenquist, Thomas A.; Sidorenko, Viktoriya S.; Iden, Charles R.; Chen, Chung‐Hsin; Pu, Yeong-Shiau; Bonala, Radha; Johnson, Francis; Dickman, Kathleen G.; Grollman, Arthur P.; Turesky, Robert J.

doi:10.1021/tx3000889

Cited by 87 publications

(201 citation statements)

References 49 publications

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“…21 Even though the amounts of AA-II present in Aristolochia herbs are usually within two- to five-fold of the amounts of AA-I, 19,70,71 the dA-AL-II adduct was detected at a frequency of only several percent and occurred at levels ~100-fold lower than the levels of dA-AL-I. 21,38,51 This DNA adduct biomarker data implicate dA-AL-I as the major genotoxic lesion in humans.…”

Section: Uplc-esi/ms3 Measurement Of Da-al-imentioning

confidence: 98%

“…38 Subsequently, stable isotopically labelled [ 15 N 5 ]-dA-AL-I and [ 15 N 3 ]-dA-AL-II were synthesized and employed for quantitative mass spectrometric measurements of these adducts. 51 Representative mass chromatograms and product ion spectra of dA-AL-I measured in the renal cortex of three patients with upper urothelial cancer from Taiwan, by UPLC-ESI/MS 3 , are shown in Figure 4. The level of adducts in the positive samples were 0.4 adducts and 5.9 adducts per 10 8 bases.…”

Section: Biomonitoring Of Al-dna Adducts In Humans: 32p-postlabeling mentioning

confidence: 99%

“…69 Of the 148 Taiwanese subjects assayed by MS, 132 subjects harbored dA-AL-I at a level above 0.3 adducts per 10 8 DNA bases (the LOQ value) in the renal cortex (unpublished data). 25,45,51 The mean level of dA-AL-I was 16.0 adducts per 10 8 DNA bases with a 95% confidence interval range from 10.1 to 21.0 adducts per 10 8 DNA bases (a value of 0.15 adducts per 10 8 DNA bases, one-half the LOQ value for non-positive samples, was used for the calculation of the 95% CI).…”

Section: Uplc-esi/ms3 Measurement Of Da-al-imentioning

confidence: 99%

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New approaches for biomonitoring exposure to the human carcinogen aristolochic acid

et al. 2015

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Aristolochic acids (AA) are found in all Aristolochia herbaceous plants, many of which have been used worldwide for medicinal purposes for centuries. AA are causal agents of the chronic kidney disease entity termed aristolochic acid nephropathy (AAN) and potent upper urinary tract carcinogens in humans. AAN and upper urinary tract cancers are endemic in rural areas of Croatia and other Balkan countries where exposure to AA occurs through the ingestion of home-baked bread contaminated with Aristolochia seeds. In Asia, exposure to AA occurs through usage of traditional Chinese medicinal herbs containing Aristolochia. Despite warnings from regulatory agencies, traditional Chinese herbs containing AA continue to be used world-wide. In this review, we highlight novel approaches to quantify exposure to AA, by analysis of aristolactam (AL) DNA adducts, employing ultraperformance liquid chromatography–electrospray ionization/multistage mass spectrometry (UPLC-ESI/MSn). DNA adducts are a measure of internal exposure to AA and serve as an important end point for cross-species extrapolation of toxicity data and human risk assessment. The level of sensitivity of UPLC-ESI/MSn surpasses the limits of detection of AL-DNA adducts obtained by 32P-postlabeling techniques, the most widely employed methods for detecting putative DNA adducts in humans. AL-DNA adducts can be measured by UPLC-ESI/MS3, not only in fresh frozen renal tissue, but also in formalin-fixed, paraffin-embedded (FFPE) samples, an underutilized biospecimen for assessing chemical exposures, and in exfoliated urinary cells, a non-invasive approach. The frequent detection of AL DNA adducts in renal tissues, combined with the characteristic mutational spectrum induced by AA in TP53 and other genes provides compelling data for a role of AA in upper urothelial tract cancer.

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Section: Uplc-esi/ms3 Measurement Of Da-al-imentioning

confidence: 98%

Section: Biomonitoring Of Al-dna Adducts In Humans: 32p-postlabeling mentioning

confidence: 99%

Section: Uplc-esi/ms3 Measurement Of Da-al-imentioning

confidence: 99%

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New approaches for biomonitoring exposure to the human carcinogen aristolochic acid

et al. 2015

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“…AL-DNA adducts may persist for over 20 years after the exposure had ceased (15, 16) and can be measured by 32 P-postlabelling (14, 17) or by ultra-performance-liquid chromatography-electrospray ionization-multistage scan mass spectrometry (UPLC-ESI-MS/MS n ), both applicable to formalin-fixed paraffin-embedded (FFPE) tissues (16, 18, 19). However, the 32 P-postlabeling method lacks specificity, and access to the UPLC-ESI-MS/MS n methodology and its optimization for biomaterial of low quantity are limiting factors.…”

Section: Introductionmentioning

confidence: 99%

Low-Coverage Exome Sequencing Screen in Formalin-Fixed Paraffin-Embedded Tumors Reveals Evidence of Exposure to Carcinogenic Aristolochic Acid

Castells

Karanović

Ardin

et al. 2015

Cancer Epidemiology, Biomarkers &Amp; Prevention

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Background Dietary exposure to cytotoxic and carcinogenic aristolochic acid (AA) causes severe nephropathy typically associated with urological cancers. Monitoring of AA exposure uses biomarkers such as aristolactam-DNA adducts, detected by mass spectrometry in the kidney cortex, or the somatic A>T transversion pattern characteristic of exposure to AA, as revealed by previous DNA sequencing studies using fresh frozen tumors. Methods Here we report a low-coverage whole-exome sequencing method (LC-WES) optimized for multi-sample detection of the AA mutational signature, and demonstrate its utility in 17 formalin-fixed paraffin-embedded urothelial tumors obtained from 15 patients with endemic nephropathy, an environmental form of aristolochic acid nephropathy. Results LC-WES identified the AA signature, alongside signatures of age and APOBEC enzyme activity, in 15 samples sequenced at the average per-base coverage of ~10x. Analysis at 3–9x coverage revealed the signature in 91% of the positive samples. The exome-wide distribution of the predominant A>T transversions exhibited a stochastic pattern whereas 83 cancer driver genes were enriched for recurrent non-synonymous A>T mutations. In two patients, pairs of tumors from different parts of the urinary tract, including the bladder, harbored overlapping mutation patterns, suggesting tumor dissemination via cell seeding. Conclusion LC-WES analysis of archived tumor tissues is a reliable method applicable to investigations of both the exposure to AA and its biologic effects in human carcinomas. Impact By detecting cancers associated with AA exposure in high-risk populations, LC-WES can support future molecular epidemiology studies and provide evidence-base for relevant preventive measures.

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“…Another important effect of kidney damage is the presence of albumin or other protein in the urine. This measurement of proteinuria is definitive but is somewhat lacking in sensitivity, so combinations of protein tests and urine creatinine are also used for assessing kidney function [99].…”

Section: Creatinine Normalization In Metabolomicsmentioning

confidence: 99%

Application of liquid chromatography-mass spectrometry and differential mobility spectrometry-mass spectrometry for detection and quantitation of biomarkers in complex biological matrices

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Biomonitoring of Aristolactam-DNA Adducts in Human Tissues Using Ultra-Performance Liquid Chromatography/Ion-Trap Mass Spectrometry

Cited by 87 publications

References 49 publications

New approaches for biomonitoring exposure to the human carcinogen aristolochic acid

New approaches for biomonitoring exposure to the human carcinogen aristolochic acid

Low-Coverage Exome Sequencing Screen in Formalin-Fixed Paraffin-Embedded Tumors Reveals Evidence of Exposure to Carcinogenic Aristolochic Acid

Application of liquid chromatography-mass spectrometry and differential mobility spectrometry-mass spectrometry for detection and quantitation of biomarkers in complex biological matrices

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