CHARACTERISATION OF DELTA-8 -THC DISTILLATES USING HPLC WITH PDA AND MASS SPECTROMETRY DETECTION
Posters | 2022 | Waters | ISCInstrumentation
Delta-8-THC has emerged as a rapid-growth cannabinoid in consumer products derived from hemp, raising safety and regulatory concerns due to its intoxicating effects and the potential presence of synthesis byproducts. Accurate characterization of Δ8-THC distillates is essential for ensuring product purity, consumer safety, and compliance with evolving regulations.
This study aims to develop and demonstrate a robust analytical workflow for the identification and quantification of Δ8-THC and related cannabinoids in distillate samples. Key goals include:
The following instrumentation and software were employed:
Samples and standards were dissolved in acetonitrile and injected (5 µL) onto the HPLC column. A binary gradient of 0.1% formic acid in water (solvent A) and acetonitrile (solvent B) delivered separation at 25 °C and 1.592 mL/min. PDA detected UV absorbance at 228 nm, while MS acquired [M+H]+ data. Unknown peaks were explored through retention time alignment, PDA spectral comparison, mass spectral matching against the in-house library, and in-source fragmentation experiments at varying cone voltages.
The neutral cannabinoid mixture baseline-separated ten compounds, including CBD, CBN, exo-THC, Δ9-THC, and Δ8-THC. Analysis of a Δ8-THC distillate revealed:
Implementing HPLC-PDA-MS with software-driven spectral library searching offers:
Advancements may include high-resolution MS for deeper structural elucidation, expanding spectral libraries to cover novel cannabinoids and byproducts, and integrating automated workflows for high-throughput quality control. Coupling ion mobility or tandem MS could further resolve co-eluting isomers and reduce false positives.
The presented HPLC-PDA-MS approach effectively separates and identifies Δ8-THC and related cannabinoid isomers in distillates. Library matching and in-source fragmentation increased identification confidence for unknown peaks. Such workflows are critical for ensuring product safety in the rapidly evolving cannabinoid market.
HPLC, LC/MS, LC/SQ
IndustriesFood & Agriculture
ManufacturerWaters
Summary
Significance of the Topic
Delta-8-THC has emerged as a rapid-growth cannabinoid in consumer products derived from hemp, raising safety and regulatory concerns due to its intoxicating effects and the potential presence of synthesis byproducts. Accurate characterization of Δ8-THC distillates is essential for ensuring product purity, consumer safety, and compliance with evolving regulations.
Objectives and Study Overview
This study aims to develop and demonstrate a robust analytical workflow for the identification and quantification of Δ8-THC and related cannabinoids in distillate samples. Key goals include:
- Separating neutral cannabinoid isomers using HPLC.
- Detecting compounds via photodiode array (PDA) and single-quadrupole mass spectrometry.
- Utilizing software tools for spectral library matching and in-source fragmentation analysis.
Instrumentation Used
The following instrumentation and software were employed:
- ACQUITY Arc HPLC system with CORTECS C18 column (4.6×100 mm, 2.7 µm).
- 2998 PDA detector (210–400 nm, single wavelength at 228 nm).
- ACQUITY QDa single-quadrupole mass detector (ESI+, 100–800 Da, cone voltages 15 V and 45 V).
- Empower chromatography data software with a custom cannabinoid spectral library.
Methodology
Samples and standards were dissolved in acetonitrile and injected (5 µL) onto the HPLC column. A binary gradient of 0.1% formic acid in water (solvent A) and acetonitrile (solvent B) delivered separation at 25 °C and 1.592 mL/min. PDA detected UV absorbance at 228 nm, while MS acquired [M+H]+ data. Unknown peaks were explored through retention time alignment, PDA spectral comparison, mass spectral matching against the in-house library, and in-source fragmentation experiments at varying cone voltages.
Key Results and Discussion
The neutral cannabinoid mixture baseline-separated ten compounds, including CBD, CBN, exo-THC, Δ9-THC, and Δ8-THC. Analysis of a Δ8-THC distillate revealed:
- A dominant Δ8-THC peak (66 % area) at tR 5.35 min.
- Multiple minor peaks (2–12 % area) with identical [M+H]+ m/z 315, indicating possible isomeric cannabinoids eluting between 4.0 and 7.0 min.
- Successful library matching for two late-eluting unknowns at tR 6.15 min and 6.53 min.
- In-source fragmentation confirming the identity of (6aR,9R)-Δ10-THC through characteristic product ions (m/z 259, 193, 135, 123).
Benefits and Practical Applications
Implementing HPLC-PDA-MS with software-driven spectral library searching offers:
- Reliable differentiation of cannabinoid isomers in complex matrices.
- Rapid screening of Δ8-THC products for safety and regulatory compliance.
- Enhanced confidence in component identification via combined UV and mass fragmentation data.
Future Trends and Possibilities
Advancements may include high-resolution MS for deeper structural elucidation, expanding spectral libraries to cover novel cannabinoids and byproducts, and integrating automated workflows for high-throughput quality control. Coupling ion mobility or tandem MS could further resolve co-eluting isomers and reduce false positives.
Conclusion
The presented HPLC-PDA-MS approach effectively separates and identifies Δ8-THC and related cannabinoid isomers in distillates. Library matching and in-source fragmentation increased identification confidence for unknown peaks. Such workflows are critical for ensuring product safety in the rapidly evolving cannabinoid market.
References
- Erickson, B.E. C&En News. “Delta-8-THC craze concerns chemists,” 2021.
- Hudalla, C. The Cannabis Scientist. “We believe in unicorns (and Delta-8),” 2021.
- Webster, G.R.B. et al. US Patent Appl. US20040143126A1.
- Golombek, P. et al. Toxics, 8(2), 2020.
- Kiselak, T.D. et al. Forensic Sci Int, 308, 2020.
- Meehan-Atrash, J. & Rahman, I. Chem Res Toxicol, 35(1), 2022.
- Watanabe, K. et al. Forensic Toxicology, 25(1), 2007.
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