europaea and N. multiformis, BVD-523 nmr but inhibited that of the AOA, N. maritimus (91% reduced growth rate compared with controls) and N. devanaterra (81%) (Fig. 2a, Table 1). Continuous illumination at 60 μE m−2 s−1 completely inhibited growth of the two studied AOA species, but only partially inhibited growth of AOB strains (Figs 1 and 2, Table 1). The highest light intensity (500 μE m−2 s−1) completely inhibited growth of all AOB and AOA strains. Apparent differences in sensitivity to photoinhibition of AOA species were only observed at the lowest light intensity, where N. devanaterra was less sensitive than N. maritimus. For

AOB, N. europaea was more sensitive than N. multiformis, with respective decreases in specific growth rate of 91% and 41% at 60 μE m−2 s−1 (Fig. 1, Table 1). In natural environments, diurnal cycles enable the recovery of ammonia oxidizers from photoinhibition and growth. This was therefore investigated for all strains using 8-h light/16-h dark cycles at the two lowest light intensities. At 15 μE m−2 s−1, AOB were Epigenetics Compound Library screening not significantly inhibited, as found under continuous illumination. At 60 μE m−2 s−1, however, photoinhibition was lower than that under continuous illumination. There was no significant reduction in

the specific growth rate of N. europaea, demonstrating an ability to recover during periods of darkness, while the growth of N. multiformis was reduced by only 14%, compared to 41% under continuous illumination (Fig. 1), suggesting partial recovery. Photoinhibition of N. maritimus was not influenced by light cycling, with almost complete inhibition at both light intensities. There was evidence of some recovery of growth of N. devanaterra at 60 μE m−2 s−1, where inhibition was only 63% and surprisingly lower than at 15 μE m−2 s−1 continuous illumination. Light plays a key role in the nitrogen cycle in aquatic ecosystems, stimulating uptake and excretion of inorganic nitrogen and inhibiting nitrification (Nelson & Conway, 1979; Hooper & Terry, 1973). The detrimental

effect of light on ammonia-oxidizing Histamine H2 receptor bacteria (AOB) has been known for many years. Hooper & Terry (1973, 1974) demonstrated light inhibition of ammonia oxidation by N. europaea suspended cells, with maximum inhibition at short, near-UV wavelength (410 nm). Horrigan & Springer (1990) reported variability in the photosensitivity of ammonia oxidizers such as Nitrosococcus oceanus and strain SF-2, isolated from sea-surface films, and Guerrero & Jones (1996a) provided further evidence of species-specific and dose- and wavelength-dependent photoinhibition. Results from the present study support these previous findings. Photoinhibition appears to operate on the initial step of ammonia oxidation, which is catalysed by ammonia monooxygenase.