Preselection of the Bog Butter Standards

The criteria used for identifying suitable bog butter finds for use as radiocarbon standards were (1) bog butter specimens large enough to allow up to 500 g to be sampled with minimal impact on their historical or cultural value and their overall integrity; (2) specimens that survived in several pieces (either post-excavation, at the time of discovery, or at the time of reporting) and not deemed suitable for museum display; (3) absence of conservation treatments involving organic-based products; (4) absence of modern contamination deriving from the excavation and storage (e.g. plasticizers from plastic bags); (5) lipid distribution with approximately equal abundances of C_16:0 and C_18:0 FAs (i.e. ratio C_16:0/C_18:0 as close as possible to 1) to enable the same masses of each fatty acid to be extracted and isolated during CSRA; (6) lipid distribution with relatively low abundances of C_18:1 FA or other compounds which could partially coelute with the C_18:0 (or C_16:0) FA; and (7) in cases where several specimens fulfil the above criteria, samples with significantly different dates were considered desirable.

Bog butter specimens contained in vessels were oftentimes subject to wax treatment in the past for the purposes of consolidation of the vessel. This process rendered these particular specimens unsuitable for our current purpose (criterion 3). From the remaining specimens, we identified nine of large size (> 10 kg; criterion 1) and in several pieces (criterion 2) as being the potential candidates for use as standards (Table 1). Three of them (IB4, IB20, IB29) had been previously analyzed and were not re-sampled (Smyth et al. Reference Smyth, Berstan, Casanova, McCormick, Mulhall, Sikora, Synnott and Evershed2019). At this stage, two different areas of each of the remaining bog butter specimens were sub-sampled for both lipid and radiocarbon analyses.

Table 1 Bog butter specimens preselected, bulk conventional ¹⁴C age, C_16:0/C_18:0 peak area ratio and stable carbon isotope values.

The lipid analyses by GC and GC-MS revealed all nine sampled specimens to be free of obvious contamination from storage or restoration work (criteria 3, 4). The C_14:0, C_16:0 and C_18:0 FAs were found to be dominant in the TLE of all the specimens. Some of the bog butter specimens also contained hydroxy fatty acids (OHFAs; the 10-C_18:0 OHFA being dominant), biomarkers of adipocere formation (Smyth et al. Reference Smyth, Berstan, Casanova, McCormick, Mulhall, Sikora, Synnott and Evershed2019), in appreciable abundances. Only five specimens (IB4, IB29, IB33, IB37, IB38) showed a peak area ratio of C_16:0/C_18:0 FAs below 2 (Table 1; criterion 5). Sample IB37, however, displayed significantly different C_16:0/C_18:0 FA peak area ratios between the two sub-samples with one at 1.6 and the other at 2.7, suggesting its lipid composition was inhomogeneous. Two specimens (IB29, IB34) showed the presence of C_18:1 FA at similar abundance to the C_18:0 FA, and thus were not suitable (criterion 6). The δ¹³C values on the C_16:0 and C_18:0 FAs measured by GC-C-IRMS of six specimens (IB4, IB20, IB29, IB34, IB36, IB38) plotted firmly in the reference range of ruminant dairy animals (Copley et al. Reference Copley, Berstan, Dudd, Docherty, Mukherjee, Straker, Payne and Evershed2003) and two others (IB33, IB35) at the edge of this reference range confirming that all of these specimens were dairy fats (Table 1, Figure 1a). Sample IB37, however, displayed δ¹³C_16:0/18:0 values outside the reference range of ruminant animals with one sub-sample plotting in the dairy region (Δ¹³C < –3.1‰) and the other in the ruminant adipose region (Δ¹³C > –3.1‰), thus being of uncertain origin.

Figure 1 (a) δ¹³C_18:0 values plotted against δ¹³C_16:0 values and (b) calibrated bulk radiocarbon dates (calibrated using OxCal v4.4.2 and the IntCal20 terrestrial calibration curve; Reimer et al. Reference Reimer, Austin, Bard, Bayliss, Blackwell, Ramsey, Butzin, Cheng, Edwards, Friedrich, Grootes, Guilderson, Hajdas, Heaton, Hogg, Hughen, Kromer, Manning, Muscheler, Palmer, Pearson, van der Plicht, Reimer, Richards, Scott, Southon, Turney, Wacker, Adolphi, Büntgen, Capano, Fahrni, Fogtmann-Schulz, Friedrich, Köhler, Kudsk, Miyake, Olsen, Reinig, Sakamoto, Sookdeo and Talamo2020) for the nine preselected bog butter specimens.

The bulk radiocarbon dates on the sub-samples for bog butter specimens IB33 to IB38 inclusive provided statistically consistent measurements. The radiocarbon dates identified one specimen (IB33) as dating to the Early Bronze Age, five (IB4, IB34 to IB37 inclusive) dating to the Iron Age, one (IB20) of medieval date and two (IB29, IB38) of post-medieval date (Table 1, Figure 1b).

Only three specimens, therefore, matched all the selection criteria. Specimen IB4 has a C_16:0/C_18:0 ratio of 1.85 and dates to 1924 ± 26 BP, IB33 has an average ratio of 1.55 and dates to 3765 ± 26 BP, finally, IB38 has an average ratio of 1.25 and dates to 330 ± 18 BP. Specimens IB33 and IB38 were selected as those bog butter specimens to be used as radiocarbon standards as they exhibited the smallest C_16:0/C_18:0 ratios (criterion 5). These specimens also display very distinct radiocarbon ages providing one standard in the range of prehistoric pottery vessels and another in the range of historical vessels (criterion 7).

Cleaning and Homogenization

We sampled 495.37 g of IB33 and 426.12 g of IB38 for the creation of radiocarbon standards (Figure 2 a1-2, b1-2). During the initial freeze-drying step, 17.0% of the mass of IB33, and 3.3% of the mass of IB38, were lost as water. After the removal of visible contaminants (animal hair, pieces of ancient wooden container and peat particles, stored afterwards in separate glass vials) using the melting and centrifuging process, 377.6 g (76.6% of the initial mass) of IB33 and 406.6 g (95.4% of the initial mass) of IB38 remained for homogenization (Figure 2 a3, b3).

Figure 2 Pictures of the main steps to generate homogenous radiocarbon standards from (a) IB33 and (b) IB38 bog butter finds: 1. Bog butter specimens from the NMI collections (left) and sampling with tweezers and scalpel removing obvious contaminants (e.g. pieces of wooden container) (right). 2. Sampled masses for cleaning. 3. Masses collected after removal of visible contaminants by melting and centrifuging (left), isolated peat-like contaminant materials (middle), isolated wooden materials and animal hair (right). 4. Homogenization by melting in a large beaker (left), pouring in a tray covered in foil (middle) and cooled bog butters as thin tablets (right). 5. Bog butter standards divided into eight pieces (left) and remaining material collected from the beaker and after slicing (right).

Once homogenized, cooled and solidified (Figure 2 a4, b4), the bog butter specimens were sliced into eight plates with total masses of 372.4 g (75.0% of the initial mass) and 400.6 g (94.0% of the initial mass) for IB33 and IB38, respectively (Figure 2 a5, b5). The remaining loose material account for 2.5 g (0.4% of the initial mass) and 2.9 g (0.7% of the initial mass) of IB33 and IB38, respectively. In total, 373.9 g (75.5% of the initial mass) of IB33 and 403.5 g (94.7% of the initial mass) of IB38 were homogenized and constitute the amounts of the new radiocarbon standards available. The different plates are now stored individually wrapped in foil in aluminium trays to avoid potential contamination during future handling of the standards.

Homogeneity Assessment

To assess the homogeneity in terms of lipid composition and radiocarbon age, the eight plates and the two vials of material were analyzed, resulting in a total of 10 analyses per bog butter specimen.

The lipid analyses (Table 2, Figure 3 a,b) revealed a C_16:0/C_18:0 peak area ratio average of 1.62 ± 0.03 (SD) with extreme values of 1.59 and 1.67 for IB33 and an average of 1.29 ± 0.05 (SD) with extreme values of 1.26 and 1.41 for IB38. These values are close to the original ratios and suggest the lipid profiles were not altered during the preparation procedure and the bog butter standards are homogeneous. The δ¹³C_16:0/18:0 values from the different pieces are statistically indistinguishable as the means were found to be δ¹³C_16:0 = −31.5 ± 0.1‰ and δ¹³C_18:0 = −35.6 ± 0.1‰ (T’=0.4, T’(5%) = 16.9, ν = 9 and T’ = 0.5, T’(5%) = 16.9, ν = 9, respectively) for IB33 and δ¹³C_16:0 = −29.3 ± 0.1‰ and δ¹³C_18:0 = −33.6 ± 0.2‰ (T’ = 0.3, T’(5%) = 16.9, ν = 9 and T’ = 0.9, T’(5%) = 16.9, ν = 9, respectively) for IB38 (Figure 2c). These results further support the homogeneity of the two bog butter standards.

Table 2 Results of homogenization for IB33 and IB38. Mass of pieces, ratio of C_16:0/C_18:0, stable carbon isotope analyses (analytical error is 0.5‰ and averages are reported), bulk and CSRA measurements reported as the conventional radiocarbon age. *Measurement excluded (outliers or C_16:0 and C_18:0 ages non-statistically identical).

Figure 3 GC lipid profile of (a) IB33 (plate 1) and (b) IB38 (plate 1) after homogenization. (c) δ¹³C_18:0 values plotted against δ¹³C_16:0 values after homogenization.

Both bulk and CSRA determinations were performed to assess the homogeneity in radiocarbon ages of the subsamples (Table 2). Our quality assurance criteria for the CSRA approach is to obtain statistically consistent ages at the 5% level between the two fatty acids (Casanova et al. Reference Casanova, Knowles, Williams, Crump and Evershed2018, Reference Casanova, Knowles, Bayliss, Dunne, Barański, Denaire, Lefranc, di Lernia, Roffet-Salque, Smyth, Barclay, Gillard, Claßen, Coles, Illet, Jeunesse, Krueger, Marciniak, Minnitt, Rotunno, van de Velde, van Wijk, Cotton, Daykin and Evershed2020a).

For bulk measurements on IB33, one measurement (plate 8) was detected as a statistical outlier and was re-measured. With the new date on plate 8, the bulk dates are statistically identical at the 5% level (T’ = 8.7, T’(5%) = 16.9, ν = 9) and give a weighted mean of 3777 ± 5 BP. For CSRA measurements, the C_16:0 and C_18:0 FA radiocarbon ages pass the statistical consistency test at the 5% level for all of the 10 plates and vials. The measurements on individual fatty acids are statistically consistent at the 5% level (T’ = 14.3, T’(5%) = 30.1, ν = 19) and give a weighted mean of 3776 ± 6 BP. If the C_16:0 and C_18:0 FA ages are combined for each piece prior to calculating their weighted means (as would usually be the case when reporting an age of a pottery vessel), the results are also statistically consistent (T’ = 3.8, T’(5%) = 16.9, ν = 9) and their weighted mean is 3775 ± 8 BP. For this bog butter specimen, the CSRA weighted mean age (both using individual and combined C_16:0 and C_18:0 FA measurements) is statistically indistinguishable to that obtained on bulk material (T’ = 0.0, T’(5%) = 3.8, ν = 1 for both). Taken all together, individual bulk- and CSRA measurements for the butter IB33-2016:177 are statistically indistinguishable whether using the individual (T’ = 23, T’(5%) = 42.6, ν = 29) or combined (T’ = 12.5, T’(5%) = 30.1, ν = 19) ages of the C_16:0 and C_18:0 FAs. The weighted mean was found to be 3777 ± 4 BP in both cases.

The bulk measurements on IB38 are statistically indistinguishable at the 5% level (T’ = 5.1, T’(5%) = 16.9, ν = 9) and give a weighted mean of 339 ± 4 BP. For CSRA measurements on IB38, the C_16:0 and C_18:0 FA radiocarbon ages pass the statistical consistency test at the 5% level for nine plates and vials. The CSRA of Plate 5 provided inconsistent measurements, the C_18:0 FA radiocarbon age likely being erroneous due to its older age and was re-measured. The second CSRA measurements on this plate are statistically consistent and are used in the remainder of the analyses. The measurements on individual C_16:0 and C_18:0 FAs are statistically consistent at the 5% level (T’ = 6.4, T’(5%) = 28.9, ν = 18) and their weighted mean is 334 ± 6 BP. If the C_16:0 and C_18:0 FAs for each piece are combined (as would usually be the case when reporting an age of a pottery vessel), the results are also statistically consistent (T’ = 1.8, T’(5%) = 16.9, ν = 9) and give a weighted mean of 334 ± 8 BP. The CSRA weighted means are statistically indistinguishable from the those obtained on bulk measurements ((T’ = 0.5, T’(5%) = 3.8, ν = 1 and T’ = 0.5, T’(5%) = 3.8, ν = 1 and T’ = 0.3, T’(5%) = 3.8, ν = 1 and T’ = 0.5, T’(5%) = 3.8, ν = 1 and, for the individual and combined measurements of FAs, respectively). Taken all together, individual bulk and CSRA ages determined for the bog butter specimen IB38 are statistically indistinguishable whether we use the individual (T’ = 12, T’(5%) = 42.6, ν = 29) or combined (T’ = 7.2, T’(5%) = 30.1, ν = 19) ages of the two FAs. The weighted mean was found to be 338 ± 3 BP in both cases.

These results demonstrate that the prepared bog butter specimens are homogeneous in age whether we use a bulk or a compound-specific approach. The results also confirm that no exogenous carbon is introduced during the pcGC protocol in any quantity that would significantly affect the CSRA determinations.