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Solid Phase Microextraction: Solventless Sample Preparation for Monitoring Flavor Compounds by Capillary Gas Chromatography

Guides | 1998 | MerckInstrumentation
GC, SPME, GC columns, Consumables
Industries
Manufacturer
Merck

Summary

Importance of the Topic


Solid phase microextraction (SPME) offers a rapid, solvent-free sample preparation approach critical for monitoring flavor and fragrance compounds. By minimizing sample handling and avoiding organic solvents, SPME enhances detection limits and maintains chromatographic resolution. Its simplicity and adaptability make it valuable across food, beverage, and product quality control environments.

Objectives and Overview


This article introduces SPME as an alternative to traditional extraction methods and reviews its applications in analyzing flavor and fragrance components. It aims to explain the principles of SPME, describe fiber coatings and sampling modes, demonstrate coupling with capillary gas chromatography (GC) and mass spectrometry (MS), and present representative results across diverse sample matrices.

Methodology and Sampling


SPME relies on equilibria among the sample matrix, headspace, and a coated fused-silica fiber. Analysts select fiber coatings (e.g. PDMS, PDMS/DVB, PDMS/Carboxen, Carbowax/DVB, polyacrylate) to match analyte polarity and volatility. Sampling modes include direct immersion for liquid-phase analytes and headspace extraction for volatile compounds, with parameters such as temperature (30–65°C), addition of salt, agitation, and sampling time (1–45 min) optimized for sensitivity. Thermal desorption in GC injectors releases analytes directly onto capillary columns without solvent interference.

Used Instrumentation


  • SPME fiber holders (manual and automated)
  • PDMS and mixed-phase SPME fibers (100 µm, 65 µm, 75 µm coatings)
  • Capillary GC columns (SPB-1, SPB-5, PTE-5, β-DEX 120, MDN-5)
  • Detectors: Flame ionization (FID), quadrupole MS, ion trap MS, TOFMS
  • Temperature-controlled sampling vials and stirring apparatus


Main Results and Discussion


SPME performance was demonstrated across multiple matrices:
  • Fruit beverages: Immersion SPME with 100 µm PDMS provided comparable or improved sensitivity versus dichloromethane extraction for esters, terpenoids, and acids in juice.
  • Whole fruits: Headspace SPME with PDMS/DVB and other fibers captured key volatiles (hexenal, hexanal, furaneol) in tomatoes, strawberries, and apples even after cold storage.
  • Flavor oils: One-minute headspace SPME quantified menthol in chocolate bars and resolved enantiomers in mint and spearmint oils using chiral columns.
  • Complex matrices: Headspace SPME eliminated glycerin interference in punch flavor samples and quantified isothiocyanates in cocktail sauce, revealing kinetic flavor losses.
  • Rancidity and off-odors: SPME detected oxidation markers (hexanal, nonanal) in oils and chips and measured 2,4,6-trichloroanisole in wine at ppt levels by focused MS scan modes.


Benefits and Practical Applications


  • Solventless, fast analysis reduces cost and hazardous waste.
  • Minimal sample handling preserves volatile profiles and lowers blank contamination.
  • Wide linear dynamic range down to parts-per-trillion concentrations.
  • Compatibility with standard GC and GC-MS systems simplifies adoption in QA/QC and research labs.


Future Trends and Potential Applications


Ongoing developments include automated SPME platforms for high-throughput screening, novel fiber coatings for broader analyte selectivity, coupling with fast GC and ambient MS techniques, and in-situ monitoring of real-time flavor release in food processing and storage.

Conclusion


SPME has emerged as a versatile and robust technique for trace-level analysis of flavor and fragrance compounds. Its simplicity, solvent-free operation, and precise quantitation make it an attractive alternative to traditional extraction methods. Continued innovation in fiber chemistry and instrumentation promises to expand its applications across food, beverage, fragrance, and environmental analysis.

References


  1. Arthur CL, Potter DW, Buchholz KD, Motlagh S, Pawliszyn J. LC/GC. 1992;10(9):656–661.
  2. Arthur CL, Killam LM, Motlagh S, Lim M, Potter DW, Pawliszyn J. Environ Sci Technol. 1992;26:979–983.
  3. Arthur CL, Pratt K, Motlagh S, Pawliszyn J. J High Resol Chromatogr. 1992;15:741–744.
  4. Arthur C, Killam L, Buchholz K, Potter D, Chai M, Zhang Z, Pawliszyn J. Environ Lab. 1992/93:10–14.
  5. Zhang Z, Pawliszyn J. Anal Chem. 1993;65:1843–1852.
  6. Yang X, Peppard T. J Agric Food Chem. 1994;42:1925–1930.
  7. Harmon A. In: Marsli R, editor. Techniques for Analyzing Food Aroma. Marcel Dekker; 1997. p 96–100.
  8. Marsili RT. J Chromatogr Sci. 1984;22:61–67.
  9. Snyder JM, Frankel EN, Selke E. JAOCS. 1985;62:1675–1679.
  10. Wyatt DM. J Chromatogr Sci. 1987;25:7–11.

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