GC/MS detection of short chain fatty acids from mammalian feces using automated sample preparation in aqueous solution
Applications | 2018 | Agilent TechnologiesInstrumentation
Short chain fatty acids (SCFAs) produced by gut microbiota play critical roles in host metabolism, immunity and disease processes. Reliable profiling of SCFAs in fecal samples supports research in microbiome–host interactions, clinical diagnostics and quality control in industrial and pharmaceutical applications.
This study describes an automated, aqueous‐phase derivatization protocol using isobutyl chloroformate and GC/MS analysis to profile C1–C7 SCFAs in mammalian feces. The goal was to overcome challenges of SCFA volatility and hydrophilicity without time‐consuming drying steps, enabling robust identification, quantitation and high throughput sample processing.
Sample Preparation
Derivatization
All analyses were performed on an Agilent 7890B GC coupled to a 5977B single‐quadrupole MSD and equipped with a 7693A autosampler. Key parameters included:
Chromatographic Separation
The optimized isobutylation chemistry achieved clear separation of 14 SCFAs, including formic through heptanoic acid. Derivatization reagent peaks at ~6.5 and 14.3 min did not interfere with analytes.
Calibration and Linearity
Excellent linearity (R² ≥ 0.996) was obtained over picogram to nanogram on-column masses, accommodating high natural variability of C1–C4 versus C5–C7 SCFAs.
Sample Profiling
Human and feline fecal samples consistently showed high acetic (C2), propionic (C3) and butanoic (C4) acid levels, with acetic acid dominating. The automated protocol enabled rapid profiling across multiple samples.
Ongoing developments may include coupling with high-resolution MS for expanded metabolite coverage, miniaturized sample preparation for single‐cell and low-biomass studies, and integration with data-driven microbiome–metabolome correlation analyses. Advances in greener reagents and microfluidic automation will further streamline SCFA profiling.
This work presents a robust, automated aqueous derivatization GC/MS method for comprehensive SCFA profiling in fecal samples. The protocol achieves excellent sensitivity, linearity and throughput without solvent drying, positioning it for broad application in metabolomics and clinical laboratories.
GC/MSD, GC/SQ
IndustriesMetabolomics, Clinical Research
ManufacturerAgilent Technologies
Summary
Importance of the Topic
Short chain fatty acids (SCFAs) produced by gut microbiota play critical roles in host metabolism, immunity and disease processes. Reliable profiling of SCFAs in fecal samples supports research in microbiome–host interactions, clinical diagnostics and quality control in industrial and pharmaceutical applications.
Study Objectives and Overview
This study describes an automated, aqueous‐phase derivatization protocol using isobutyl chloroformate and GC/MS analysis to profile C1–C7 SCFAs in mammalian feces. The goal was to overcome challenges of SCFA volatility and hydrophilicity without time‐consuming drying steps, enabling robust identification, quantitation and high throughput sample processing.
Methodology
Sample Preparation
- Fresh fecal aliquots (100–150 mg) homogenized with 10% isobutanol in water.
- Phase separation using NaOH and chloroform to remove lipids and contaminants.
- Addition of internal standard (3‐methylpentanoic acid) to monitor recovery.
- Volume adjustment and boiling chip added to minimize foaming.
Derivatization
- Direct reaction with 50 µL isobutyl chloroformate in aqueous medium.
- Release of CO₂ facilitated by open‐lid reaction, followed by vortexing and hexane extraction.
- Centrifugation to obtain derivatized SCFAs in the organic phase for GC/MS injection.
Instrumentation
All analyses were performed on an Agilent 7890B GC coupled to a 5977B single‐quadrupole MSD and equipped with a 7693A autosampler. Key parameters included:
- Column: VF-5ms (30 m × 0.25 mm, 0.5 µm).
- Injection: split 50:1 at 260 °C.
- Oven program: 40 °C (5 min), 10 °C/min to 310 °C.
- MS detection: scan m/z 30–350; source 250 °C, quad 150 °C.
Main Results and Discussion
Chromatographic Separation
The optimized isobutylation chemistry achieved clear separation of 14 SCFAs, including formic through heptanoic acid. Derivatization reagent peaks at ~6.5 and 14.3 min did not interfere with analytes.
Calibration and Linearity
Excellent linearity (R² ≥ 0.996) was obtained over picogram to nanogram on-column masses, accommodating high natural variability of C1–C4 versus C5–C7 SCFAs.
Sample Profiling
Human and feline fecal samples consistently showed high acetic (C2), propionic (C3) and butanoic (C4) acid levels, with acetic acid dominating. The automated protocol enabled rapid profiling across multiple samples.
Benefits and Practical Applications
- Aqueous derivatization eliminates drying steps, reducing sample loss and improving accuracy.
- Integration with an autosampler supports fully automated workflows for routine and high-throughput analyses.
- Versatile platform suitable for clinical research, microbiome studies, QA/QC in food and pharmaceutical industries.
Future Trends and Opportunities
Ongoing developments may include coupling with high-resolution MS for expanded metabolite coverage, miniaturized sample preparation for single‐cell and low-biomass studies, and integration with data-driven microbiome–metabolome correlation analyses. Advances in greener reagents and microfluidic automation will further streamline SCFA profiling.
Conclusion
This work presents a robust, automated aqueous derivatization GC/MS method for comprehensive SCFA profiling in fecal samples. The protocol achieves excellent sensitivity, linearity and throughput without solvent drying, positioning it for broad application in metabolomics and clinical laboratories.
References
- Matsumoto M. et al. Impact of intestinal microbiota on intestinal luminal metabolome. Scientific Reports 2012;2(233):1–10.
- Primec M., Mičetić-Turk D., Langerholc T. Analysis of short-chain fatty acids in human feces: A scoping review. Anal Biochem 2017;526:9–21.
- Olsen M.A., Mathiesen S.D. Production rates of volatile fatty acids in the minke whale forestomach. Br J Nutr 1996;75:21–31.
- Pons A. et al. Sequential GC/MS Analysis of Sialic Acids, Monosaccharides, and Amino Acids of Glycoproteins as Heptafluorobutyrate Derivatives. Biochemistry 2003;42:8342–8353.
- Hallmann C., van Aarssen B.G.K., Grice K. Relative efficiency of free fatty acid butyl esterification. J Chromatogr A 2008;1198–1199:14–20.
- Zheng X. et al. A targeted metabolomic protocol for short-chain fatty acids and branched-chain amino acids. Metabolomics 2013;9(4):818–827.
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