Combining collagen extraction with mineral Zn isotope analyses from a single sample for robust palaeoecological investigations
McCormack, J., Bourgon, N., Sinet-Mathiot, V., Rezek, Z., Smith, G. M.
It is advisable to refer to the publisher's version if you intend to cite from this work. See Guidance on citing. To link to this item DOI: 10.1007/s12520-022-01601-7 Abstract/SummaryCollagen extraction from bones or dentine, commonly used for radiocarbon (14C) dating and stable carbon and nitrogen isotope (δ13C and δ15N) analyses, involves the dissolution of the bioapatite of skeletal elements. This fraction is typically disposed of during pretreatment. Here, we test the possibility of utilising this dissolved mineral solution for analysis of the bioapatite zinc isotope composition (δ66Zn). Bioapatite δ66Zn is a novel trophic level indicator similar to collagen δ15N but with isotopic fractionation independent from nitrogen, thus providing additional dietary information. We tested ways to minimise Zn contamination of the dissolved mineral phase during collagen extraction. We then used archaeological bone samples from Ain Difa (Jordan) and Ranis (Germany) to compare δ66Zn values of dissolved bioapatite following our col�lagen extraction protocol with δ66Zn values from the same sample material dissolved in a metal-free cleanroom. Our results demonstrate that with only minor adjustments to minimise Zn contamination, the dissolved mineral solution from collagen extraction protocols commonly employed for 14C dating and (palaeo)dietary analysis can be used for additional δ66Zn analy�ses even when collagen extraction does not take place in a cleanroom. Our protocol allows us to gain an additional dietary proxy to complement δ15N trophic level interpretations and perform more robust (palaeo)ecological investigations without further destructive sampling.
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