AbstractThe stable carbon isotope composition (δ13C) of plant components such as plant wax biomarkers is an important tool for reconstructing past vegetation. Plant wax δ13C is mainly controlled by photosynthetic pathways, allowing for the differentiation of C4 tropical grasses and C3 forests. Proxy interpretations are however complicated by additional factors such as aridity, vegetation density, elevation, and the considerable δ13C variability found among C3 plant species. Moreover, studies on plant wax δ13C in tropical soils and plants have focused on Africa, while structurally different South American savannas, shrublands and rainforests remain understudied. Here, we analyze the δ13C composition of long‐chain n‐alkanes and fatty acids from tropical South American soils and leaf litter to assess the isotopic variability in each vegetation type and to investigate the influence of climatic features on δ13C. Rainforests and open vegetation types show distinct values, with rainforests having a narrow range of low δ13C values (n‐C29 alkane: ‰ ; Suess‐effect corrected). This allows for the detection of even minor incursions of savanna (δ13C n‐C29 alkane ‰) into rainforests. While Cerrado savannas and semi‐arid Caatinga shrublands grow under distinctly different climates, they can yield indistinct δ13C values for most compounds. Cerrado soils and litter show pronounced isotopic spreads between the n‐C33 and n‐C29 alkanes, while Caatinga shrublands show consistent values across the two homologs, thereby enabling the differentiation of these vegetation types. The same multi‐homolog isotope analysis can be extended to differentiate African shrublands from savannas.
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