18O-labelled water (GOP)

Template:BreadcrumbsPrimaryProduction

Gross oxygen production
Approach: stable isotope tracer (¹⁸O-water)
Context: incubation, in situ
Spatial scale: point sample
Temporal scale: hours to one day
Units: µmol O₂ L^-1 d^-1; convertible to µmol C L^-1 d^-1
Community captured: all
Co-measurements: initial dissolved O₂ concentration; photosynthetic quotient (PQ) for C conversion; parallel O₂/Ar measurement for respiration by difference

Method Overview

H₂¹⁸O is added to seawater incubations, enriching the water isotopically. During oxygenic photosynthesis, phytoplankton split water molecules, releasing O₂ that carries the ¹⁸O label. The accumulation of ¹⁸O₂ above natural abundance is measured by isotope ratio mass spectrometry (IRMS) at the end of the incubation, and the rate of ¹⁸O₂ production is converted to gross oxygen production (GOP)^[1].

Unlike the ¹⁴C method, the ¹⁸O approach directly measures gross O₂ production before respiratory consumption. Combined with a simultaneous measurement of net O₂ exchange (e.g., via O₂/Ar), community respiration can be estimated by difference.

Scale of measurement

Each incubation provides a point measurement. Standard incubations run for hours to one day. The small sample volume (~50 mL) limits the approach to discrete sampling rather than continuous deployment.

Data generated

The primary output is the gross O₂ production rate. Conversion to gross carbon fixation requires the photosynthetic quotient (PQ, mol O₂ produced per mol CO₂ fixed, typically 1.1–1.4 depending on substrate and nitrogen source).

Units & currency

Units are µmol O₂ L^-1 d^-1, or µmol C L^-1 d^-1 after PQ conversion. The primary currency is oxygen; carbon is the derived currency.

Sample size

Typical samples are ~50 mL in volume.

Repositories & databases

Limitations

The method assumes that newly produced ¹⁸O₂ mixes rapidly and uniformly with the dissolved O₂ pool in the incubation vessel. Light-dependent O₂ consumption (Mehler reaction, photorespiration) can cause overestimation of gross carbon fixation when rates are converted via PQ. Bottle confinement effects apply. Small sample volumes exclude larger, rarer phytoplankton.

Example Applications & Protocols

Classic examples

Bender et al. (1987) A comparison of four methods for determining planktonic community production ^[1]

Recent applications

Common calculations/conversions

GOP (µmol O₂ L^-1 d^-1) = (¹⁸O excess in POO / ¹⁸O enrichment of water) × [O₂]_initial / incubation time.
Gross C fixation = GOP / PQ.

References

↑ ^1.0 ^1.1 Bender, M., Grande, K., Johnson, K., Marra, J., Williams, P. J. le B., Sieburth, J., Pilson, M., Langdon, C., Hitchcock, G., Orchardo, J., Hunt, C., Donaghay, P., & Heinemann, K. (1987). A comparison of four methods for determining planktonic community production. Limnology and Oceanography, 32(5), 1085–1098. https://doi.org/10.4319/lo.1987.32.5.1085

[Bender1987-1] 1.0 ^1.1 Bender, M., Grande, K., Johnson, K., Marra, J., Williams, P. J. le B., Sieburth, J., Pilson, M., Langdon, C., Hitchcock, G., Orchardo, J., Hunt, C., Donaghay, P., & Heinemann, K. (1987). A comparison of four methods for determining planktonic community production. Limnology and Oceanography, 32(5), 1085–1098. https://doi.org/10.4319/lo.1987.32.5.1085

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