Biofluid Metabolomics and Lipidomics of Mice Exposed to External Very High-Dose Rate Radiation

Evan L Pannkuk; Evagelia C Laiakis; Guy Garty; Shivani Bansal; Brian Ponnaiya; Xuefeng Wu; Shanaz A Ghandhi; Sally A Amundson; David J Brenner; Albert J Fornace Jr

doi:10.3390/metabo12060520

Biofluid Metabolomics and Lipidomics of Mice Exposed to External Very High-Dose Rate Radiation

Metabolites. 2022 Jun 4;12(6):520. doi: 10.3390/metabo12060520.

Authors

Evan L Pannkuk^{1

2

3}, Evagelia C Laiakis^{1

2

3}, Guy Garty^{4

5}, Shivani Bansal¹, Brian Ponnaiya⁵, Xuefeng Wu⁵, Shanaz A Ghandhi⁵, Sally A Amundson⁵, David J Brenner⁵, Albert J Fornace Jr^{1

2

3}

Affiliations

¹ Department of Oncology, Lombardi Comprehensive Cancer Center, Georgetown University Medical Center, Washington, DC 20057, USA.
² Department of Biochemistry and Molecular & Cellular Biology, Georgetown University Medical Center, Washington, DC 20057, USA.
³ Center for Metabolomic Studies, Georgetown University, Washington, DC 20057, USA.
⁴ Radiological Research Accelerator Facility, Columbia University, Irvington, NY 10032, USA.
⁵ Center for Radiological Research, Columbia University Irving Medical Center, New York, NY 10032, USA.

Abstract

High-throughput biodosimetry methods to determine exposure to ionizing radiation (IR) that can also be easily scaled to multiple testing sites in emergency situations are needed in the event of malicious attacks or nuclear accidents that may involve a substantial number of civilians. In the event of an improvised nuclear device (IND), a complex IR exposure will have a very high-dose rate (VHDR) component from an initial blast. We have previously addressed low-dose rate (LDR, ≤1 Gy/day) exposures from internal emitters on biofluid small molecule signatures, but further research on the VHDR component of the initial blast is required. Here, we exposed 8- to 10-week-old male C57BL/6 mice to an acute dose of 3 Gy using a reference dose rate of 0.7 Gy/min or a VHDR of 7 Gy/s, collected urine and serum at 1 and 7 d, then compared the metabolite signatures using either untargeted (urine) or targeted (serum) approaches with liquid chromatography mass spectrometry platforms. A Random Forest classification approach showed strikingly similar changes in urinary signatures at 1 d post-irradiation with VHDR samples grouping closer to control samples at 7 d. Identical metabolite panels (carnitine, trigonelline, xanthurenic acid, N6,N6,N6-trimethyllysine, spermine, and hexosamine-valine-isoleucine-OH) could differentiate IR exposed individuals with high sensitivity and specificity (area under the receiver operating characteristic (AUROC) curves 0.89-1.00) irrespective of dose rate at both days. For serum, the top 25 significant lipids affected by IR exposure showed slightly higher perturbations at 0.7 Gy/min vs. 7 Gy/s; however, identical panels showed excellent sensitivity and specificity at 1 d (three hexosylceramides (16:0), (18:0), (24:0), sphingomyelin [26:1], lysophosphatidylethanolamine [22:1]). Mice could not be differentiated from control samples at 7 d for a 3 Gy exposure based on serum lipid signatures. As with LDR exposures, we found that identical biofluid small molecule signatures can identify IR exposed individuals irrespective of dose rate, which shows promise for more universal applications of metabolomics for biodosimetry.

Keywords: biodosimetry; ionizing radiation; lipidomics; mass spectrometry; metabolomics; very high-dose rate.

Abstract

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