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Radiocarbon dating of lipids preserved in pottery vessels: guidelines for best-practice in compound-specific 14C analyses

Published online by Cambridge University Press:  02 August 2024

Emmanuelle Casanova*
Affiliation:
Organic Geochemistry Unit, School of Chemistry, University of Bristol, Cantock’s Close, Bristol, BS8 1TS, UK
Timothy D J Knowles
Affiliation:
Organic Geochemistry Unit, School of Chemistry, University of Bristol, Cantock’s Close, Bristol, BS8 1TS, UK Bristol Radiocarbon Accelerator Mass Spectrometry Facility, University of Bristol, 43 Woodland Road Bristol, BS8 1UU, UK
Alex Bayliss
Affiliation:
Scientific Dating, Historic England, Cannon Bridge House, 25 Dowgate Hill, London, EC4R 2YA, UK
Richard P Evershed
Affiliation:
Organic Geochemistry Unit, School of Chemistry, University of Bristol, Cantock’s Close, Bristol, BS8 1TS, UK Bristol Radiocarbon Accelerator Mass Spectrometry Facility, University of Bristol, 43 Woodland Road Bristol, BS8 1UU, UK
*
Corresponding author: Emmanuelle Casanova; Email: emmanuelle.casanova@lsce.ipsl.fr
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Abstract

Pottery vessels played a central role in the processing, storage and transport of animal and plant products by prehistoric and historic peoples with their chemical residues surviving for thousands of years. Accurate radiocarbon dating of archaeological pottery vessels by isolating reliable sources of carbon relating to the use of pots has long been a major challenge, but is now possible using compound-specific radiocarbon analysis of absorbed organic residues preserved in the ceramic fabric of the vessel wall. This method involves the radiocarbon dating of single fatty acids most commonly derived from degraded animal fats. These compounds are extracted from the ceramic matrix and isolated from potentially interfering compounds using preparative capillary gas chromatography. When coupled with lipid biomarker and compound-specific stable carbon isotope analyses, this method enables the palaeodietary and chronological information contained in archaeological lipids preserved in ceramic vessels to be interpreted together. From a practical perspective the methodology is challenging and for successful application must adhere to rigorous protocols. We present here guidelines which include (i) consideration of pottery selection, (ii) technical parameters for the isolation of fatty acids then their 14C dating and calibration, and (iii) case studies selected to illustrate the best use of this method.

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Type
Conference Paper
Creative Commons
Creative Common License - CCCreative Common License - BY
This is an Open Access article, distributed under the terms of the Creative Commons Attribution licence (http://creativecommons.org/licenses/by/4.0/), which permits unrestricted re-use, distribution and reproduction, provided the original article is properly cited.
Copyright
© The Author(s), 2024. Published by Cambridge University Press on behalf of University of Arizona
Figure 0

Figure 1 Photographs of potsherds from the early Neolithic sites of a. Rosheim “Rittergass”, France and b. Robin Hood Ball, UK with examples of 1. Refitting potsherds, 2. Non-refitting potsherds judged to be from the same vessel, 3. Single decoratively (a. Linearbandkeramik decoration) or typologically (b. carinated bowl) characteristic potsherds, and 4. Single undecorated potsherds.

Figure 1

Figure 2 Partial gas chromatograms of potsherds with concentrations suitable for 14C dating for a. ROS-C-4694 b. ROS-C-4682 c. ROS-C-4701 d. ROS-C-4677 exhibiting “pure” animal fats and various ratios of the C16:0 and C18:0 fatty acids, e. ROS-C-4615 showing a mixture of animal fat and beeswax and f. ROS-C-4617 showing a dominance of beeswax. IS is the internal standard and numbers corresponds to the carbon chain lengths of the various alkyl lipids.

Figure 2

Table 1 Table showing the numbers of potsherds: analyzed per site, containing animal fats, with concentration >500 µg.g-1, and suitable for 14C dating for the overall assemblage, refitted, decorated and undecorated sherds. The percentages are calculated for the total number of sherds per category except for the bold values that are the percentage of the total number of sherds analyzed per site. BIS = Bischoffsheim, ROS = Rosheim, COL = Colmar, ENS = Ensisheim, SIE = Sierentz, LBK = Linearbandkeramik (early Neolithic), Gro. = Grossgartach (Middle Neolithic), Roe. = Roessen (Middle Neolithic)

Figure 3

Figure 3 a. Main steps of the pretreatment procedure: i. Cleaning of potsherd surface ii. Extraction of lipids from powdered ceramic on heating block iii. Solventless trapping system for isolation of single compounds by pcGC. b. Gas chromatograms of potsherd lipid extracts suitable for 14C dating (upper) with the dashed lines indicating the trapping windows required to isolate C16:0 and C18:0 fatty acids, and the contents of the waste traps after isolation by pcGC (lower).

Figure 4

Table 2 F14C of C16:0 and C18:0 FA dated directly and after methylation and pcGC isolation. F14CFA corresponds to the fatty acid, F14CFAME to the fatty acid after methylation, F14CFA.1 to the correction of additional methyl group using mass balance calculation, and F14CFA.2 to the correction of the methyl group using the refined correction to account for fractionation

Figure 5

Figure 4 a. Compilation of reference values of modern ruminant adipose, ruminant dairy, porcine adipose fats, marine and freshwater species from the UK, Libya and Kazakhstan (Copley et al. 2003; Cramp and Evershed 2014; Dunne et al. 2012; Outram et al. 2009). Ellipses represent the 68% (1σ) of the values. b,c. Percentage of marine products in the lipid extracts expressed as probability distributions (b) box and whisker plots (c) for the potsherds BN74 and BN89. d. Calibration of reference terrestrial animal bone dates and the dates on the lipids from potsherd BN74 and BN89 uncorrected and corrected for the marine reservoir effect (From Casanova et al. 2020b).