4 and 5, respectively. The matrices shown here are representative for optimal growth conditions (low to medium light intensity depending on species, nutrient replete growth media and sampled during the exponential growth phase). The F 0 fluorescence matrices show prominent fluorescence JNJ-26481585 clinical trial emission features in cyanobacteria under orange-red excitation that are characteristic
of PBS (fluorescence emission around 650 nm from allophycocyanin) and Chla (680 nm) pigments. In contrast, the algal strains reflect the absorption MRT67307 mouse of light by chlorophylls and carotenoids in the blue-green spectral region with a sharply defined emission related to Chla fluorescence. Fig. 4 F 0 excitation–emission matrices of a culture of each of the species included in this study. These cultures were sampled under nutrient replete growth conditions and had F v/F m values of 0.6–0.7. The matrices are normalized to the spectral maximum to facilitate LY2603618 molecular weight comparison
of spectral differences between the different species Fig. 5 F v/F m excitation–emission matrices for the cultures shown in Fig. 4 Despite the sharp distinction in F 0 profiles observed between algae and cyanobacteria, F v/F m matrices (Fig. 5) show relatively constant F v/F m in the Chla emission band in both cyanobacteria and algae. For algal fluorescence, the variable component extends along the whole excitation spectrum for emission from ~650 to at least 750 nm (the maximum measured). The excitation–emission patterns for the cyanobacterial cultures show a smoother transition from low to high F v/F m when emission wavelength increases towards the maximum of PSII Chla (680–690 nm), but a sharp drop of F v/F m at longer emission wavelengths (>700 nm). These features
can respectively be explained by a variable component to PBS fluorescence (discussed further below), and the allocation of most Chla molecules to the non-variable PSI in cyanobacteria (Johnsen and Sakshaug 1996, 2007). The feature-rich F v/F m profile of cyanobacteria implies that the spectral location and bandwidth of emission detection can have a major Phenylethanolamine N-methyltransferase influence on readings of F v/F m, when we target Chla emission in cyanobacteria. Optimization of detector slit spectral position and bandwidth for equivalent readings of F v/F m in cyanobacteria and algae are discussed in more detail below. Simulations of community fluorescence F v/F m is used to assess the maximum efficiency of PSII in dark-acclimated cells. F v/F m can be expressed for all waveband pairs in the excitation/emission matrix, and because the fluorescence excitation–emission matrices of algae and cyanobacteria differ prominently (Fig.