In situ simultaneous measuring method for the determination of key processes of soil organic carbon cycling: Soil microbial respiration using laser spectrometry

IF 3 Q2 CHEMISTRY, ANALYTICAL Analytical science advances Pub Date : 2023-12-26 DOI:10.1002/ansa.202300054
Hongzhao Yuan, Zhen He, Liping Zhang, Jiurong Wang, Zhenke Zhu, Tida Ge
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Abstract

Rationale: Soil microbial heterotrophic C-CO2 respiration is important for C cycling. Soil CO2 differentiation and quantification are vital for understanding soil C cycling and CO2 emission mitigation. Presently, soil microbial respiration (SR) quantification models are based on native soil organic matter (SOM) and require consistent monitoring of δ13C and CO2.

Methods: We present a new apparatus for achieving in situ soil static chamber incubation and simultaneous CO2 and δ13C monitoring by cavity ring-down spectroscopy (CRDS) coupled with a soil culture and gas introduction module (SCGIM) with multi-channel. After a meticulous five-point inter-calibration, the repeatability of CO2 and δ13C values by using CRDS-SCGIM were determined, and compared with those obtained using gas chromatography (GC) and isotope ratio mass spectrometry (IRMS), respectively. We examined the method regarding quantifying SR with various concentrations and enrichment of glucose and then applied it to investigate the responses of SR to the addition of different exogenous organic materials (glucose and rice residues) into paddy soils during a 21-day incubation.

Results: The CRDS-SCGIM CO2 and δ13C measurements were conducted with high precision (< 1.0 µmol/mol and 1‰, respectively). The optimal sampling interval and the amount added were not exceeded 4 h and 200 mg C/100 g dry soil in a 1 L incubation bottle, respectively; the 13C-enrichment of 3%–7% was appropriate. The total SR rates observed were 0.6–4.2 µL/h/g and the exogenous organic materials induced -49%–28% of priming effects in native SOM mineralisation.

Conclusions: Our results show that CRDS-SCGIM is a method suitable for the quantification of soil microbial CO2 respiration, requiring less extensive lab resources than GC/IRMS.

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测定土壤有机碳循环关键过程的原位同步测量方法:利用激光光谱仪测定土壤微生物呼吸作用
理由:土壤微生物异养 C-CO2 呼吸对 C 循环非常重要。土壤二氧化碳的分化和量化对于了解土壤碳循环和减少二氧化碳排放至关重要。目前,土壤微生物呼吸(SR)量化模型基于原生土壤有机质(SOM),需要对δ13C 和 CO2 进行持续监测:方法:我们介绍了一种新型仪器,该仪器通过空腔环降光谱仪(CRDS)与带多通道的土壤培养和气体导入模块(SCGIM)相结合,实现了原位土壤静态室培养以及二氧化碳和δ13C的同步监测。经过细致的五点相互校准后,确定了利用 CRDS-SCGIM 监测 CO2 和 δ13C 值的重复性,并分别与利用气相色谱法(GC)和同位素比质谱法(IRMS)获得的值进行了比较。我们检验了该方法对不同浓度和富集度葡萄糖的 SR 的定量分析,然后将其用于研究在 21 天的培养过程中,SR 对稻田土壤中添加不同外源有机物(葡萄糖和稻米残渣)的反应:结果:CRDS-SCGIM 的 CO2 和 δ13C 测量精度很高(分别为 1.0 µmol/mol 和 1‰)。最佳取样间隔和添加量分别不超过 4 小时和 200 毫克碳/100 克干土壤(1 升培养瓶);13C 富集度为 3%-7% 为宜。观察到的总SR速率为0.6-4.2 µL/h/g,外源有机物对本地SOM矿化的启动效应为-49%-28%:我们的研究结果表明,CRDS-SCGIM 是一种适用于土壤微生物二氧化碳呼吸定量的方法,与 GC/IRMS 相比,它所需的实验室资源更少。
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