Extended Data Table 3 Growth of MK-D1 after incubation of 120 days with a range of substrates
From: Isolation of an archaeon at the prokaryote–eukaryote interface

- A dash indicates that data were not taken for that sample.
- aThe iTAG analysis was performed for samples in which an increase of about 10 times or more in 16S rRNA gene copy numbers of MK-D1 was observed after incubation; data were analysed by qPCR assay. Detailed results are shown in Supplementary Table 1.
- bFinal concentration of casamino acids was 0.05% (w/v).
- cFinal concentration of each amino acid was 0.1 mM.
- dPowdered milk for baby (Hohoemi, Meiji) was used at a final concentration of 0.1% (w/v).
- eThe concentration of hydrogen gas was in the head space of the culture bottle.
- f2-BES was added to inhibit methanogens.
- gAddition of nitrate completely suppressed the growth of MK-D1. This is probably because nitrate inhibits formate dehydrogenase activity of MK-D195.
- hArchaeal cell membrane components were a mixture of phytol, intact polar lipid–glycerol-dialkyl-glycerol tetraethers and core lipid– glycerol-dialkyl-glycerol tetraethers (each at a final concentration 50 ng ml−1). We used the archaeal membrane components as these have a positive effect on the growth of some archaeal species: (i) archaeal cell extract including membrane lipids stimulates the growth of the extremely thermophilic archaeon Thermocaldium modestius96, and (ii) the hyperthermophilic archaeon Thermofilum pendes requires the polar lipids for growth, which was obtained from the archaeal species Thermoproteus tenax97.