Optimization of variable fluorescence measurements of phytoplankton communities with cyanobacteria

Excitation–emission fluorescence matrices of phytoplankton communities were simulated from laboratory-grown algae and cyanobacteria cultures, to define the optical configurations of theoretical fluorometers that either minimize or maximize the representation of these phytoplankton groups in community variable fluorescence measurements. Excitation sources that match the photosystem II (PSII) action spectrum of cyanobacteria do not necessarily lead to equal representation of cyanobacteria in community fluorescence. In communities with an equal share of algae and cyanobacteria, inducible PSII fluorescence in algae can be retrieved from community fluorescence under blue excitation (450–470 nm) with high accuracy (R 2 = 1.00). The highest correlation between community and cyanobacterial variable fluorescence is obtained under orange-red excitation in the 590–650 nm range (R 2 = 0.54). Gaussian band decomposition reveals that in the presence of cyanobacteria, the emission detection slit must be narrow (up to 10 nm) and centred on PSII chlorophyll-a emission (~683 nm) to avoid severe dampening of the signal by weakly variable phycobilisomal fluorescence and non-variable photosystem I fluorescence. When these optimizations of the optical configuration of the fluorometer are followed, both cyanobacterial and algal cultures in nutrient replete exponential growth exhibit values of the maximum quantum yield of charge separation in PSII in the range of 0.65–0.7.


Introduction
Differences in pigmentation are used to discriminate taxonomic phytoplankton groups in applications ranging from microscopy to remote sensing of water colour. The highest level of pigment discrimination between phytoplankton groups is found between prokaryotic cyanobacteria and the vast majority of algal taxa. Chlorophylls and carotenoids are dominant in algae, while phycobilipigments (phycoerythrin, phycoerythrocyanin, phycocyanin and allophycocyanin) are the main light harvesting pigments in cyanobacteria (prochlorophytes excepted) and red algae. Phycobilipigments extend the absorption of light to the green-orange part of the visible spectrum that is left unused by the algal groups. This spectral domain overlaps with the deepest penetration of solar irradiance in inland and coastal waters where turbidity and/or the concentration of coloured dissolved organic matter is high, yielding an advantage in light-harvesting at depth to phycobilin-containing species (Pick 1991;Stomp et al. 2007).
Owing to the differences in pigmentation between the major phytoplankton groups, absorption and fluorescence techniques can be used to interpret biomass at the community and sub-community level (Yentsch and Yentsch 1979;Kolbowski and Schreiber 1995;Beutler et al. 2002;Millie et al. 2002;Beutler et al. 2003;Seppälä and Olli 2008). In vivo chlorophyll a (Chla) fluorescence is a widely used proxy of phytoplankton biomass, a non-intrusive measurement that can be carried out with high spatial resolution (Lorenzen 1966;Kiefer 1973) under the assumption that the Chla fluorescence yield is constant. When excited with blue light, Chla fluorescence per unit concentration in cyanobacteria tends, however, to be up to an order of magnitude lower than in algae, which results in erroneous biomass estimates unless corrected for (Vincent 1983;Seppälä et al. 2007). The distribution of Chla between photosystems I and II (PSI, PSII) is fundamentally different in these phytoplankton groups Sakshaug 1996, 2007), and requires consideration in all aspects of phytoplankton community fluorescence measurements.
Variable fluorescence methods relate the rise of fluorescence that occurs with 'closure' of PSII centres under saturating illumination to energy flow in PSII (Kautsky and Hirsch 1931;Genty et al. 1989). Closed reaction centres cannot use the energy absorbed in the photosystem antennae for photochemistry and emit at least part of the excess energy as fluorescence (e.g. Gilmore and Govindjee 1999). Saturating light conditions can be induced by generating intense light pulses, such as used in pulse-amplitude modulation (PAM), pump-and-probe and fast-repetition rate fluorescence (FRRF) techniques. These methods are designed to measure both the minimum (F 0 , before closure of the reaction centres and after dark-adapting the sample) and maximum inducible (F m , reaction centres closed) level of fluorescence. The variable (inducible) part of fluorescence is expressed as F v = F m -F 0 , and when normalized to F m (F v /F m ) presents a measure of the maximum quantum yield of charge separation at PSII. Under ambient light conditions, the operational quantum yield of PSII (F v 0 /F m 0 ) is obtained instead. Both parameters are useful as they respond to nutrient limitation, excess light or transiently when growth conditions change. A combination of darkand light adapted measurements can be used to determine the electron transport rate under known irradiance(s), which can in turn be used to model primary production (Kolber and Falkowski 1993). The current work focuses on the experimental manipulation and spectral measurement of dark-adapted F v /F m . The use of this parameter in higher level applications is discussed at length in recent reviews of literature on the subject (Suggett et al. 2004, Huot andBabin 2010).
Advances in light-emitting diode (LED) manufacturing have led to the availability of narrow-band, high-power excitation light sources of high efficiency and stability. Their rapid flash capability and high output makes them the light source of choice for FRRF protocols and for PAM applications that require a small footprint. In FRRF, microsecond flashlets provide a saturating flash train within a single turnover period of PSII (\100-150 ls). PAM-type fluorometers have been developed with a combination of light sources of different colours for some time. FRRF instruments were until very recently limited to the use of LEDs of one colour in order to produce sufficiently bright flashlets. Blue light sources have been chosen to provide overlap with the absorption by Chla and accessory photosynthetic pigments in algae, but do not overlap with cyanobacterial phycobilipigment absorption (Johnsen and Sakshaug 2007). Recent studies have shown that blue-light equipped FRRF instruments are relatively insensitive to the presence of cyanobacteria, if these do not possess shortwavelength forms of phycoerythrin (Raateoja et al. 2004;Suggett et al. 2004). While F v /F m can be recorded from cyanobacteria using blue excitation as long as the light source can saturate PSII, the intensity of the fluorescence is relatively low compared to algae. Variable fluorescence of cyanobacteria can alternatively be assessed from orange or red excitation sources that excite the phycobilipigments in cyanobacteria (Schubert et al. 1989). Now that LEDs are available at the brightness required by FRRF instruments, this concept stands to be adapted to the FRRF range of instrumentation. Studies on the optimization of the variable fluorescence measurement towards unbiased representation of the phytoplankton community, are therefore overdue.
In this study, we address the representation of cyanobacteria and algae in community (variable) fluorescence measurements with special emphasis on narrow-band excitation sources. Our focus is on cyanobacteria with a pigment profile that results in low fluorescence under blue light. Most coastal and freshwater cyanobacteria belong to this group, whereas common clear-water species that produce phycourobilin-rich forms of phycoerythrin have stronger fluorescence with blue excitation. We analyse fluorescence excitation-emission matrices of cultures that are subjected to various treatments of light and nutrient availability. These fluorescence matrices are used to simulate variable fluorescence of mixed algal and cyanobacterial communities from which statistical analyses of the relation between community and subcommunity variable fluorescence follows. We describe the optimal optical configuration (excitation-emission waveband pairs) to obtain F v /F m values that represent a community cross section regardless of the share of cyanobacteria in the community. The excitation-emission waveband pairs that result in the best correspondence of community F v /F m measurements with either the cyanobacterial or the algal subpopulation are also determined.
In previous studies, healthy cyanobacteria have reported maximum F v /F m in the order of 0.3-0.5 and seldom [0.6 (Raateoja et al. 2004;Suggett et al. 2009). This is markedly lower than reported for algae (0.65) and higher plants (near 0.8). Low F v /F m in healthy cells can be a measurement artefact when the light source does not provide sufficient intensity to saturate PSII (Raateoja et al. 2004). The solution is then to be found in the use of excitation wavebands that better match the photosynthetic action spectrum of the sample. It has also been suggested that phycobilipigment fluorescence can elevate F 0 in the PSII Chla fluorescence band, and thus reduce observed F v /F m (Campbell et al. 1996(Campbell et al. , 1998. Interestingly, this latter effect prevails under excitation with blue light, which incites only weak fluorescence from phycobilisome (PBS) pigments. To resolve this issue, we use Gaussian band decomposition of fluorescence emission spectra to determine the extent to which PSII F 0 and F m are offset by phycobilipigment fluorescence. We then show how the excitation and emission slits of the fluorometer can be optimized to exclude fluorescence from phycobilisomal and PSI pigments, yielding cyanobacterial F v /F m values in the same range as observed in algae.

Phytoplankton cultures
The algal species included in this study were the chlorophyte Brachiomonas submarina TV15 and the diatom Thalassiosira pseudonana TV5 from the Tvärminne culture collection (TV, University of Helsinki, Hällfors and Hällfors 1992). Cyanobacterial strains included the closely related phycocyanin-rich and phycoerythrin-rich picocyanobacteria strains Synechococcus sp. CCY9201 and CCY9202 (Culture Collection Department of Marine Microbiology, NIOO-KNAW, The Netherlands), both isolated from the Baltic Sea (Ernst et al. 2003). Further, two morphologically and optically highly similar strains of the filamentous bloom-forming Nodularia spumigena were included: strain HEM from University of Helsinki, Microbiology division (Sivonen et al. 1989), and one with an undocumented culturing history that we conservatively annotate Nodularia sp. from the TV collection. All species are common in the Baltic Sea.
Nutrient replete cultures were grown on sterile modified BG-11 media with salinity adjusted to the Baltic Sea at 8.3 g NaCl L -1 , pH = 7.4, and added vitamin B12 (0.02 lg L -1 ). Silicate was added to the diatom cultures at 0.044 g Na 2 SiO 3 Á5H 2 O L -1 . BG11 medium is rich in nitrate (N:P approximately 100:1), so cultures that were left to grow and age in a particular batch were expected to eventually become starved of phosphorous. To induce nitrogen starvation instead, selected cultures were periodically refreshed with medium with reduced (10%) nitrate (N treatment) or no nitrate (-N treatment). These treatments were expected to induce fixation of elemental nitrogen in the Nodularia strains. Light conditions were 12/12 h light/ dark from fluorescent tubes at low/medium/high light treatments of 20, 70 or 350 lmol photons m -2 s -1 , respectively, using green filters to mimic the Baltic Sea environment in the low and medium light levels. The green filters also increased production of phycobilipigments, particularly in the Synechococcus strains. The cultures were kept in suspension by daily gentle mixing, and bubbling with filtered air for 15 min every hour. The complete combination of treatments and sampling times (i.e. aging of the cultures) is presented in Table 1. Cultures that exhibited no growth after up to 2 weeks were removed from the experiment. Cultures that underwent significant visual changes were sampled more than once. The different treatments resulted in a total of 31 sampling events of cyanobacterial cultures and 15 sampling events of the algal cultures.

Absorption measurements
Spectrophotometric measurements were carried out using a PerkinElmer (Waltham, MA, USA) model Lambda650 spectrophotometer equipped with a 150-mm integrating sphere. The samples were placed in a 10-mm quartz cuvette at the front entrance of the sphere. Cultures were diluted as necessary to measure in the range where optical density (OD) was linear with dilution. In this configuration, the measured OD can be assumed proportional to absorption and backscattering. A baseline equal to OD at 800 nm was subtracted to correct for backscatter. Purified, filtered water was used as a blank reference. Absorption (a) was derived from the OD measurements using a(k) = 2.303 9 OD bc (k)/0.01, where the factor 2.303 serves to convert from a 10-based to a natural logarithm, OD bc (k) is the baseline-corrected OD at wavelength k, and 0.01 is the path length of the cuvette in meters.

Fluorescence measurements
All spectral fluorescence measurements were carried out after placing samples in low light (\10 lmol photons m -2 s -1 ) for at least 0.5 h. Excitation/emission matrices of fluorescence were recorded for the diluted (see below) samples in a 10-mm quartz cuvette in a Varian Cary Eclipse (Agilent, Santa Clara, CA, USA) fluorometer. Emission was scanned from 600 to 750 nm at 1-nm intervals and 10-nm band width, while excitation was produced with a Xenon flash lamp in 10-nm bands, at 10-nm intervals from 400 to 650 nm. It is essential for the proper determination of F v /F m that our F 0 measurements were not disturbed by fluorescence induction in any part of the excitation-emission matrix, particularly in the case of cyanobacteria which are known to undergo state transitions at very low light intensity. The excitation beam was attenuated to 25% using neutral density filter as a precaution. A selection of cultures tested before the start of the experiment showed that increasing the attenuation of the excitation light did not change the observed F v /F m or the spectral shape of F 0 emission. Repeated excitationemission matrix measurements also gave identical results. This empirical evidence, although circumstantial, suggests that neither the intensity nor the period of illumination prevented the measurement of F 0 or F v /F m . These assumptions are also supported in a theoretical sense, when we consider properties of the excitation light source and sample placement: the Xenon flash lamp produces 2-5 ls half-width pulses at 80 Hz. This flash interval ([12 ms) allows relaxation of PSII between flashes. With a microspherical PAR sensor in the focused excitation beam centred in a 10-nm wide band at 420 nm (the peak wavelength of the lamp), we derived a photon density in the order of 0.01 lmol photons m -2 flash -1 which should not excite above F 0 (see Biggins and Bruce 1989;Babin et al. 1995). Finally, the excitation beam illuminated approximately 6% of the cell suspension at any given time, while the sample was continuously stirred. These considerations support our assumption that no significant build-up of fluorescence above F 0 occurred, and that multiple turnover did not induce transitions to state I. Indeed, the placement of neutral density filter was in all likelihood not required. F m was measured by treating the samples with 3-(3,4-dichlorophenyl)-1,1-dimethylurea (DCMU, Sigma-Aldrich) to a final concentration of 30 lM. By blocking the electron acceptor side of PSII, DCMU causes a fluorescence rise to F m . Excitation-emission matrices were quantum-corrected following Kopf and Heinze (1984), accounting for spectral dependency of the light source and detector, and corrected for the spectral attenuation of the neutral density filter. The spectral resolution and detector sensitivity allowed scanning of one excitation-emission matrix in approximately 10 min. Blank spectra (culture medium) were measured daily and subtracted from F 0 and F m spectra.

Dilutions and normalization
The fluorescence data used in our analyses was normalized to absorption to correct for differences in cell density and pigmentation between cultures. The normalization was achieved by diluting the stock cultures instead of scaling measured fluorescence intensities. While this approach may cause some dilution errors, it also minimizes the effects of multiple scattering and reabsorption of fluoresced light that may be present in dense cultures. Variability in the Chlaspecific absorption at 675 nm is fairly limited in algal cultures compared to cyanobacteria, because the latter exhibit more prominent overlap between phycobilipigment and Chla absorption in the red spectral domain. In contrast, variability around the blue Chla absorption peak is relatively limited in cyanobacteria cultures and introduced foremost by photoprotective carotenoids. To prevent these differences in pigmentation from creating biases in our fluorescence data set, we used different absorption measures for the dilution of either group. The dilution target for algal cultures was set at a(675) = 5.0 m -1 . Cyanobacterial samples were diluted to match a(437) = 9.9 m -1 , which resulted in an average The numbers under each growth regime indicate the time (days) that the respective culture was left to grow/age after inoculation, before sampling took place. Growth light intensities (values in column headers) have units lmol photons m -2 s -1 . Nitrogen additions are indicated with ?N, N, -N for nitrogen replete, nitrogen limited and nitrogen deplete conditions a Ernst et al. (2003) b Sivonen et al. (1989) c Hällfors and Hällfors (1992) a(675) of 4.6 and standard deviation of 1.1 m -1 over all cyanobacteria cultures. The fluorescence signals obtained from the cultures diluted in this way were not scaled further and are henceforth referred to as fluorescence normalized to a(675) or absorption-normalized fluorescence. In a few cases where the stock culture had a lower OD than the target value, corresponding fluorescence values were proportionally adjusted. All dilutions were made using BG-11 growth medium lacking nitrate and phosphate to avoid replenishment of nutrient-starved cultures. Community fluorescence excitation-emission matrices (F 0 , F m , and derived F v /F m ) were constructed by addition of the absorption-normalized fluorescence signals.

Spectral characteristics of absorption and fluorescence
Gradual nutrient starvation, variable light exposure and sampling at various moments during culturing led to considerable variability in absorption and fluorescence. This variability is illustrated in Fig. 1 for spectral absorption and in Fig. 2 for fluorescence excitation with Chla emission measured at 683 nm. For each species that was included in our analysis Fig. 1 shows the absorption spectra of the extreme cases, in terms of the blue-to-red absorption ratio. These absorption spectra correspond to the same diluted samples that were used to measure fluorescence (Fig. 2). Samples of Synechococcus sp. CCY9202 show the characteristic absorption peak of phycoerythrin (around 560 nm) as their dominant accessory pigment. The other cyanobacteria cultures showed dominant accessory photosynthetic pigment absorption at longer wavelengths, in Nodularia matching the absorption characteristics of phycocyanin possibly mixed with phycoerythrocyanin (600-630 nm). Phycocyanin (*615 nm) showed as the dominant pigment in Synechococcus sp. CCY9201. The absorption by accessory photosynthetic pigments chlorophyll b (*650 nm) and chlorophyll c (*630 nm) can be recognized in the red part of absorption spectra of respectively the chlorophyte Brachiomonas submarina and the diatom Thalassiosira pseudonana. The range of variation in spectral absorption in algae and cyanobacteria cultures was comparable in terms of the extremes shown in Fig. 1a, b, respectively. Nevertheless, the cyanobacteria cultures were more evenly spread between these extremes than the algae cultures. High light (350 lmol m -2 s -1 ) treatment resulted in increased blueto-red absorption ratios in the algae cultures, possibly due to the enhanced production of photoprotective pigment absorbing blue light. All cyanobacteria responded to low (20 lmol m -2 s -1 ) light treatment with increased pigment production and pronounced absorption features of the phycobilipigments. Chlorosis occurred in the cyanobacteria cultures under high light treatment and increasingly with nitrogen starvation. Nodularia sp. is known to fix elemental nitrogen and its accessory pigment production appeared to recover after an initial period of reduced absorption and slow growth under nitrogen starvation. Synechococcus sp. CCY9202, adapted to low light environments (Wood 1985;Pick 1991), only showed increasing absorption under low light, while all other cyanobacteria showed prominent accessory pigment features under both low and medium light intensity (70 lmol m -2 s -1 ).
The fluorescence excitation spectra for Chla fluorescence given in Fig. 2 (as F 0 (k ex ,683)) can be interpreted as photosynthetic absorption spectra of PSII. A large difference in the blue versus red light harvesting for PSII is apparent between algae and cyanobacteria when comparing absorption in Fig. 1 to the PSII fluorescence in Fig. 2. The prominent role of Chla in light harvesting for PSII in algae, visible in the blue around 440 nm, is nearly absent in the cyanobacterial strains, where only a small share of Chla is connected to PSII Sakshaug 1996, 2007). The algal species further reveal light harvesting for PSII in the area of maximum absorption by accessory pigments in the 460-480 nm range: fluorescence resulting from excitation at 470-480 and at 650 nm in B. submarina may be attributed to Chlorophyll b, whereas in T. pseudonana, excitation at 460-470 and 630 nm would be due to Chlorophyll c and excitation at 530-540 nm due to fucoxanthin. Between the two algal species, affinity for red light was higher in B. submarina, in some cases exceeding fluorescence from red excitation found in cyanobacterial cultures that were nutrient starved. The Chla fluorescence excitation features found in the cyanobacterial cultures matched the absorption peaks of phycobilipigments given above. Between the cyanobacterial cultures Nodularia showed the highest absorption-normalized fluorescence under blue illumination. Cyanobacteria with urobilin-rich phycoerythrin, which may absorb short-wavelength light down to 490 nm and are common in clear water environments, were not included in our data set.
The variability in F v /F m of the species used in this study is shown as histograms in Fig. 3. The excitation bands to describe F v /F m in algae and cyanobacteria were selected to match peak areas in the excitation spectra (Fig. 2). F v /F m of the algae is shown for excitation at 470 nm, cyanobacterial F v /F m at 590 nm (both for 10-nm bandwidth). The emission was measured at 683 nm (10-nm bandwidth) for both groups. Maximum F v /F m in the order of 0.65 are common in phytoplankton studies (but see Samson et al. 1999;Suggett et al. 2004;Vredenberg et al. 2009). The majority of cultures included in our analyses showed F v /F m in the 0.45-0.65 range, while the range of F v /F m in cyanobacterial cultures was wider (0.1-0.7) than that of algal cultures (0.4-0.7). The top range of these F v /F m values measured in cyanobacteria exceed those commonly found in literature, where values for healthy cultures are usually in the 0.3-0.5 range (but see Raateoja et al. 2004;Suggett et al. 2009). Lower F v /F m in cyanobacteria has been attributed to incomplete saturation of PSII in FRRF studies (Raateoja et al. 2004), and to dampening of the variable fluorescence by an offset of F 0 caused by fluorescing phycobilipigments (Campbell et al. 1996(Campbell et al. , 1998, which is discussed further below. Spectral fluorescence excitation and emission properties of the phytoplankton strains used in this study are further illustrated by excitation-emission F 0 and F v /F m matrices in Figs. 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   and Chla (680 nm) pigments. In contrast, the algal strains reflect the absorption of light by chlorophylls and carotenoids in the blue-green spectral region with a sharply defined emission related to Chla fluorescence. 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 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 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. 5) it is useful to inspect excitation-emission matrices of phytoplankton communities in search of features that can be uniquely attributed to specific phytoplankton groups. This analysis requires knowledge of the spectral fluorescence properties as well as the inducible fluorescence of all species represented in a community. These requirements cannot be met when analysing natural samples consisting of multiple species contributing unique signals to bulk fluorescence. Instead, we simulated community fluorescence from the excitation-emission F 0 and F m measurements of individual cultures. We constructed community fluorescence excitation-emission matrices, each consisting of a single algal and a single cyanobacterial species. Different culturing conditions and different times of sampling (Table 1) resulted in 15 algal and 31 cyanobacterial input matrices and 465 unique combinations. With this large number of combined excitation-emission matrices for which F 0 and F m (and thus F v /F m ) were available, it was possible to perform statistical analyses of the relation between community and algal or cyanobacterial F v /F m . This evaluation was carried out for individual excitationemission waveband pairs. Although F v /F m can be measured for any waveband pair in an excitation-emission matrix, we can only interpret the variable fluorescence that originates from Chla in PSII (at 680-690 nm) in terms of the electron flux that fuels photosynthesis. We therefore examine the simulated community F v /F m excitation-emission matrices against the PSII Chla F v /F m values of their algal and cyanobacterial fractions. To identify the contribution from the algal or cyanobacterial fraction F v /F m to community F v /F m , the reference excitation-emission pair (both denoted k ref ) for cyanobacteria and algae are chosen from regions of the excitation spectrum of Chla fluorescence where we encounter a high fluorescence yield and strong variable fluorescence. We selected k ref = 470 and 590 nm of 10-nm width for algae and cyanobacteria, respectively. Choosing different k ref values within the blue and orange-red excitation domain does not lead to significantly different results. The 470-nm band is located between the absorption maxima of Chla and accessory chlorophylls in the algal cultures, the latter are not present in cyanobacteria. The 590-nm band (10-nm wide) is chosen to excite cyanobacterial phycobilipigments that absorb in the 550-630 nm domain. The emission waveband for the reference F v /F m is centred at 683 nm and has a width of 10 nm.
Owing to the large number of simulated communities, we are able to highlight the influence of algal and cyanobacterial signals in community F v /F m (k ex ,k em ) using regression statistics. The matrices of the coefficient of determination (R 2 ) of community F v /F m (k ex ,k em ) against F v /F m (k ref ,683) of their algal and cyanobacterial subpopulations are given in Fig. 6. Three excitation/emission regions (marked 1-3 in Fig. 6 and subsequent figures) are identified as showing a correlation between community, and algal or cyanobacterial F v /F m that is higher than in adjacent areas: -Region 1 shows R 2 close to 1 between community and algal F v /F m (and consequently a R 2 near 0 with the cyanobacterial fraction), under blue excitation in a wide emission band that includes Chla fluorescence and extends into the range of mixed PSI/PSII fluorescence at near-infrared wavelengths. -Region 2 is for excitation near 600 nm and emission in the Chla fluorescence band near 683 nm and returns R 2 above 0.5 for cyanobacteria but 0.2 for algae. In contrast to the correlation with algae in region 1, the excitation range with a high correlation for cyanobacterial F v /F m does not extend into the near-infrared. -Region 3, similarly to region 2, is found under orange/ red excitation, but in the emission range of phycobilipigments (620-650 nm). In this spectral domain, R 2 is greater than 0.4 for cyanobacteria and near 0 for algae, as no algal pigments fluoresce around 650 nm (Fig. 4).
While the presence of highly fluorescent phycobilipigments in cyanobacteria explains strong fluorescence between 600 and 650 nm, the correlation (R 2 [ 0.4) to variable fluorescence from PSII Chla is not straightforward, as it has commonly been assumed that phycobilipigment fluorescence is not variable (but see discussion below, and Küpper et al. 2009;Kana et al. 2009). We note that the presence of algae in the community does not influence this result as regression of F v /F m (590,650) against F v /F m (590,683) yields the same correlation when measured from the 31 individual cyanobacterial cultures.
To find optimal excitation and emission pairs for the separation of cyanobacterial and algal F v /F m in communities, we inspect the data more closely along the emission and excitation lines linked to the previously identified regions 1-3. The PSII Chla emission line (683 nm, Fig. 7a) reveals that the strongest correlations of F v /F m (k ex ,683) with algal and cyanobacterial F v /F m occurred upon excitation between 440-500 and 590-630 nm, respectively. The 470-nm excitation line (Fig. 7b) reveals that F v / F m (470,k em ), particularly for emission [650 nm, was exclusively and strongly correlated with the algal fraction of the community. The emission spectrum along the 590-nm excitation line (Fig. 7c) confirms that emission around 650 and 683 nm was best correlated with cyanobacterial F v /F m (with R 2 in the range 0.4-0.5) and weakly correlated with algal F v /F m in the Chla emission band (R 2 \ 0.2).
The data underlying the optimal excitation/emission pairs identified from Figs. 6 and 7 are presented in Fig. 8 with corresponding regression statistics. Figure 8a confirms that community F v /F m (470,683) is strongly driven by the algal F v /F m and was highly insensitive to the fluorescence of the cyanobacteria in the simulated communities. Only the case for equal absorption in the algal and cyanobacterial subpopulations is shown here, but when the community composition was skewed to 90% in favour of the cyanobacteria, community F v /F m (470,683) remained a good (relative error \10%) predictor of algal F v / F m (470,683) in 92% of cases. The fluorescence emission of the cyanobacterial fraction was too low at this excitation/ emission pair to influence community variable fluorescence, even when mixed with algal cultures of low (variable) fluorescence.
Under red-orange illumination centred at 590 nm (Fig. 8b) we note a better correlation of community and cyanobacterial F v /F m (R 2 = 0.54). The relatively low slope and high offset of this regression were clearly caused by the inclusion of cases where cyanobacterial subpopulations with low F v /F m were mixed with algae with higher F v /F m , a result of a wider spread of F v /F m in the cyanobacterial cultures compared to the algae (Fig. 3). The regression results for the algal fraction under emission at 590 nm were clearly worse with R 2 = 0.18.
The variable fluorescence originating from PBS pigments (F v /F m (590,650)) was lower than F v /F m (590,683) while the relation between community and cyanobacterial F v /F m was strong for cyanobacteria cultures with F v /F m [0.42 (Fig. 8c). Cultures with lower F v /F m included several where phycobilipigments were bleached (primarily in high light) or broken down (primarily under nitrogen stress). If these cultures are not considered, the R 2 value for cyanobacteria improved from 0.45 to 0.76. These results suggest a tight coupling between the F v /F m from PBS Emission wavelength (nm) pigments and PSII Chla, which is further explored in the next section. The high amount of scatter in the results comparing community F v /F m (590,650) against the algae fraction provides further indication that the variable fluorescence of cyanobacteria cultures can be observed from community F v /F m without interference from the presence of algae.
The nature of cyanobacterial fluorescence in the Chla emission band The emission spectra of algal cultures at room temperature have a predictable shape because their main source of fluorescence is Chla located in PSII and to a much smaller extent in PSI. In cyanobacteria, we observe fluorescence in the red spectral domain from (1) PSII Chla (variable), (2) PBS fluorescence (weakly variable) and (3) PSI (non-variable), where the contribution of the latter is relatively strong in cyanobacteria compared to algae. The role of PSI fluorescence in the red spectral domain is likely to be important in fluorometers that record fluorescence [700 nm (discussed below). The role of accessory PSII pigment composition on fluorescence in the PSII Chla emission band and towards shorter wavelengths has received very little attention altogether and is explored here. It has been suggested that phycobilipigments have a significant effect on the F 0 signal that is otherwise attributed to Chla (e.g. Campbell et al. 1996Campbell et al. , 1998. A nonvariable fluorescence source elevates F 0 and F m equally, which leads to dampening of F v /F m . We observed in the previous exercise that the PBS fluorescence does have a (weakly) variable component, which in turn should alleviate this dampening. To quantify the influence of PBS fluorescence on the variable fluorescence from PSII it is necessary to isolate F 0 and F m of the individual pigments. We decomposed F 0 and F m emission spectra of our cyanobacteria cultures into Gaussian band contributions of phycobilipigments and Chla. The Gaussian decomposition allows us to express F v /F m of each pigment component.
Emission spectra were taken from the excitation-emission matrices of all cultures used in the simulations described in the previous section. We restrict ourselves to fluorescence emission between 625 and 690 nm, assuming that components of PSI and PSII that fluoresce at longer wavelengths (PSII Chla at 730-740 nm, PSI Chla [700 nm, c.f. Ley 1980) have minimal influence in the area around 680 nm. The emission band corresponding to excitation at 590 nm (10-nm bandwidth) was selected as it yields high fluorescence in all cyanobacteria cultures. The choice or width of the excitation band does not influence the shape of the emission spectrum, as long as the excitation band overlaps with the absorption domain of the PBS pigments that fuel PSII. An overview of the boundary conditions for fitting the model is given in Table 2. Each Gaussian curve was defined as where F denotes the fluorescence at waveband k, and a the magnitude, b the centre wavelength, and c the standard deviation of the curve. We assumed no change in the value of b and c between F 0 and F m for any given sample. The least squares difference between measured F 0 or F m (625-690 nm) and the fluorescence of three pigment components (phycocyanin, allophycocyanin and Chla) was minimized, allowing up to 2.5% deviation of the fit at the pigment fluorescence maxima. Fitted spectra of N. spumigena HEM and Synechococcus sp. 9201 are presented in Fig. 9 (590,683), respectively. a-c correspond to the key excitation-emission pairs highlighted with numerical markers in Fig. 6. a F v /F m (470,683), sensitive to algal but not cyanobacterial (590,683), with stronger correspondence to cyanobacterial compared to algal F v /F m and c F v /F m (590,650), strongly related to cyanobacterial F v /F m (590,683) [0.4. Colours and symbols correspond to Fig. 7, drawn black lines mark unity. The discrete distribution of the subcommunity F v /F m values is caused by the limited number of cultures used to simulate community F v /F m matrices N. spumigena HEM (Fig. 9a, b) clearly show the variable component of fluorescence from allophycocyanin. In Synechococcus (Fig. 9c, d), it was less obvious, but present, while the overlap of PBS pigment fluorescence with Chla fluorescence was stronger.
When F v /F m data are interpreted in terms of the quantum yield of charge separation in PSII, we assume that observed F v /F m originates fully from Chla located in PSII. This concept is challenged in cyanobacteria where PBS pigment and Chla fluorescence may overlap. Using the Gaussian components of F 0 and F m , we can express the variable fluorescence of [F v /F m ] Chla which is the 'true' F v /F m that is related to electron transport in PSII. The variable fluorescence that is actually observed is referred to as [F v /F m    The two latter effects are illustrated in Fig. 10 Influence of detector band width and spectral location on retrieval of F v /F m The signal-to-noise ratio of a fluorometer improves with increasing width of the emission slit. In addition, shifting the detection band to longer wavelengths reduces cross talk from the excitation source, which becomes important when excitation includes longer wavelengths (e.g. to excite cyanobacterial pigments). The variable fluorescence from cyanobacteria is sharply peaked at the PSII Chla emission band, in contrast to algae (Figs. 5, 7c). The emission detection band width must therefore be sufficiently narrow to retain sensitivity to the optical feature. The effect of the emission bandwidth and spectral location on observed F v /F m is illustrated in Fig. 11. F v /F m (590,k em ) and F v /F m (470,k em ) of cyanobacteria and algae cultures, respectively, were normalized to their peak and plotted as a function of k em between 620 and 750 nm, and for emission band widths ranging 10-50 nm. These spectra are highly conserved between all algae (Fig. 11a), with standard deviation of normalized F v /F m spectra \10% for wavelengths [665 nm (at shorter wavebands coupling of different accessory pigments to PSII introduces some variability). In cyanobacteria (Fig. 11b), the peak of F v /F m (590,k em ) was sharply defined near the 683-nm peak of PSII Chla emission, with fluorescence from PBS pigments contributing to lower F v /F m on the short wavelength side. At wavelengths [683 nm, non-variable fluorescence from PSI pigments dampens F v /F m . Consequently, the observed F v /F m is strongly dependent on the emission detection band centre and width. For broad detection bands positioned [700 nm, the deviation from the maximum F v /F m amounted to up to 35%, equivalent to the reduction of F v /F m = 0.65 as observed for some of our cyanobacteria cultures (Fig. 3) to 0.42. The use of instruments with longpass filters with a cut-off [700 nm can thus explain low F v /F m readings in cyanobacteria, complementary to the explanation that phycobilipigment fluorescence elevates F 0 as highlighted by Campbell et al. (1998).

Interpretation of community F v /F m from selected optical configurations
We have demonstrated the need for careful selection of excitation and emission bands in fluorometer design to prevent bias against cyanobacterial representation in the measured signal. We now show some examples of community F v /F m measurements using theoretical fluorometer configurations, using the same simulated community fluorescence data as in preceding exercises. Because we use DCMU instead of illumination-induced F m in all simulations, differences in the retrieval of algal or cyanobacterial F v /F m do not reflect the (in)ability of the fluorometer to incite the maximum attainable variable fluorescence. Community F v /F m is, as before, compared to algae-and cyanobacteria-specific F v /F m (470,683) and F v /F m (590,683), respectively. The excitation bandwidth is indicated for each case, while the emission is recorded in a 10-nm wide band centred at 683 nm, i.e. the optimum setting that allows for cyanobacterial F v /F m values up to the same level as found in algae.
Results for narrow-band (10 nm) single excitation channel configurations with excitation at 470 and and b against the ratio of allophycocyanin-to-Chla F 0 . Fluorescence of the individual pigment components was assessed by Gaussian decomposition of F 0 and F m emission spectra with excitation at 590 nm 590 nm were already detailed in Fig. 8a, b, respectively. The results for the 470-nm channel configuration (Fig. 8a) were representative of excitation channels throughout the 450-500 nm range (not shown). This configuration is representative of variable fluorescence fluorometers with a filter design similar to those used for the determination of Chla concentration (excitation in the 400-500 nm range, e.g. Corning 5-60 type filter, emission with a high-pass filter [650 nm, e.g. Corning 2-64 filter). Towards longer excitation wavelengths, the representation of cyanobacterial F v /F m increases gradually, first for cultures that produce phycoerythrin and followed by phycocyanin-rich cultures. The 590-nm excitation configuration featured in Fig. 8b is representative of configurations with excitation in the 590-630 nm range, which are not individually shown here. At longer excitation wavelengths [630 nm, fluorescence in both cyanobacteria and algal groups is increasingly excited so that the signal becomes less specific to the cyanobacterial subpopulation. Moving the excitation source from 590 towards 650 nm increases the fluorescence yield in both groups (Fig. 7c), which can be explained by the presence of phycocyanin in all cyanobacterial cultures and the accessory chlorophylls b and c in the algal cultures. The absorption shoulder of Chla around 625 nm and the main red peak of Chla at 675 nm also increasingly absorb light when the excitation waveband is moved beyond 600 nm (Sathyendranath et al. 1987;Bidigare et al. 1990;Ficek et al. 2004). The relatively high affinity for illumination [600 nm in both algae and cyanobacteria implies that the light source need not be as bright to fully saturate PSII in all organisms, and error properties of the F v /F m measurement improve slightly, compared to illumination around 590 nm. At the same time, shorter wavebands prevent crosstalk between excitation and emission bands, an important consideration in fluorometer design.
Results for a fluorometer with broad-white (400-650 nm, spectrally neutral) illumination are given in Fig. 12a. This 'cool white' excitation light resulted in a weak representation of cyanobacterial F v /F m against improved results for algal cultures compared to k ex = 590 nm (Fig. 8b).
Excitation in the 535-585 nm domain should lead to approximately equal representation of algae and cyanobacteria, based on the data shown thus far. Figure 12b shows the result for such a 'broad-green' light source. The configuration is still more sensitive to algae than cyanobacteria, but the difference in regression slopes and offsets could at least in part be attributed to the presence of more cases with low F v /F m in the group of cyanobacteria, while scatter is approximately equal for both groups. Cultures of cyanobacteria with low F v /F m (and F 0 ) had limited influence on community F v /F m , especially when paired with healthy algae. For the purpose of identifying community photosynthetic capacity rather than differentiation of algal and cyanobacterial subpopulations, this is not a poor result: phytoplankton that contributes little to community photosynthesis has a proportionally lower impact on community F v /F m . This is particularly useful when one is limited to the use of a single-channel fluorometer. This configuration is of special interest because the light source targets exclusively light uptake by accessory photosynthetic pigments in both algae and cyanobacteria (i.e. not Chla), which may render community F v /F m more sensitive to changes in the accessory pigment composition, and thus to environmental conditions.

Discussion
Cyanobacteria species that are considered harmful due to the production of toxins, odorous compounds, surface scums, or benthic mats, are widespread in coastal and inland water bodies, particularly in eutrophic systems (e.g. Hallegraeff 1993;Anderson et al. 2002). Blooms of these species negatively impact ecosystem value. Monitoring the presence and activity of cyanobacteria is therefore a pressing matter in environmental policy. The distinct absorption and fluorescence properties of cyanobacteria caused by the prominent role of phycobilipigments in photosynthetic light harvesting are already used to complement traditional observation methods (e.g. microscope counts) in environmental monitoring (Lee et al. 1994;Izydorczyk et al. 2005;Seppälä et al. 2007). Variable fluorescence measurements are increasingly included in these monitoring efforts, to reveal spatiotemporal trends in photosynthetic capacity or even photosynthetic activity of the phytoplankton. FRRF instruments equipped with a series of excitation sources are increasingly becoming available, and can be used to determine both the quantum yield of photochemistry and the functional absorption cross-section of PSII at e.g. blue, green and orange or red wavelengths. With these instruments it is possible to better assess the role of phytoplankton that efficiently harvest green and orange light in aquatic photosynthesis in environments where terrigenous organic matter skews the available radiation towards the green part of the light spectrum. Such knowledge may be used to determine ecophysiological constraints of coastal and freshwater phytoplankton, but in a wider sense also help to better represent the role of light uptake in ecosystem models that focus on the environments most exposed to, and most important to, human activities. This progress in FRRF design is made possible through more efficient light sources and detectors that have become available in recent years. It is therefore timely to conceive what properties the optimal instrument for these environments should possess and what pitfalls might be avoided.
Some properties of cyanobacterial fluorescence emission must be taken into account when deciding upon the optimal detection waveband of the fluorometer, and before interpreting fluorescence induction results obtained with different fluorometer configuration. The major light harvesting pigments for photosynthesis in cyanobacteria are organized in the PBS which holds a group of highly fluorescent phycobilipigments. As long as these pigments are organized in the PBS, energy from phycoerythrin and phycocyanin will be transferred towards the core of the PBS where allophycocyanin subsequently fluoresces in the 650-670 nm range. It therefore stands to reason that this spectral domain should be avoided in fluorescence induction measurements where Chla fluorescence is used as a proxy of energy flowing through PSII. Long wavelength ([690 nm) fluorescence from PSI is also relatively strong in cyanobacteria. Regardless of the excitation band that is used we therefore find that narrow (10-nm) wavebands centred at the PSII Chla emission band (680-690 nm) yield best results (Fig. 11).
The efficiency of energy transfer from the PBS to reaction centres is considered very high (Sidler 1994 for a review), but not all harvested energy is transferred to the PSII core. Our results show PBS fluorescence in the order of 22% of F o in the Chla emission band. This emission is absent in algae (with exceptions) and theoretically leads to a lowered reading of F v /F m in cyanobacteria and in communities with a high cyanobacterial biomass (Campbell et al. 1996(Campbell et al. , 1998. We find, however, that a variable component to PBS fluorescence can alleviate the theoretical dampening of F v /F m considerably (Fig. 10). Indeed, the peak of F v /F m in the excitation-emission spectrum is found in the order of 0.65-0.75, for several cyanobacteria species (Fig. 3) Fig. 12 Simulated community F v /F m as a function of algal and cyanobacterial F v /F m , for fluorometers with different light source configurations and a 10-nm wide emission band centred at 683 nm. a A neutral white light source (400-650 nm), b a broad-green light source (535-585 nm) due to the overlapping fluorescence of PBS pigments and Chla. Such high F v /F m values for cyanobacteria have been reported in very few other studies (Raateoja et al. 2004;Suggett et al. 2009), which used FRRF. Variable fluorescence from PBS is surprising; it has been assumed that these pigments do not exhibit variable fluorescence at all. These findings that are reflected in some recent studies using different fluorescence induction techniques (Küpper et al. 2009;Kana et al. 2009) challenge the idea of a constant, highly efficient resonance transfer from PBS pigments to the reaction centres. Our fluorescence data provide insufficient means to explore the relation between the rise of PBS fluorescence and closing of PSII reaction centres, or to see how illumination or nutrient conditions might influence PBS F v /F m . Nevertheless, it is notable that F v /F m from the PBS at 650 nm showed a fair correlation with cyanobacterial PSII Chla F v /F m (Fig. 8c). In a pilot experiment that is not presented here, we exposed N. spumigena with saturating light flashes (590 nm) and observed induction of PBS fluorescence (650 nm), suggesting that the present result is neither merely an artefact of DCMU treatment nor to prolonged exposure to light in our spectrofluorometer. If the mechanism behind phycobilisomal variable fluorescence can be explained in terms of PSII kinetics, this may open up the way to study the physiology of cyanobacteria in natural communities. The possibility of variable fluorescence from phycobilipigments in cryptophytes and rhodophytes should in such studies be taken into account.
The excitation spectrum of fluorescence in PSII is primarily dependent on the photosynthetic pigment composition, which distinguishes the major phytoplankton groups and, with exceptions, clearly separates cyanobacteria from algae (Fig. 2). Blue-green illumination (\550 nm) excites stronger fluorescence in algal cultures than in cyanobacteria (Yentsch and Yentsch 1979;Vincent 1983;Schubert et al. 1989). Longer wavelength illumination favours cyanobacterial fluorescence but algal fluorescence remains significant. If the emission band is located at its optimum of 680-690 nm, as we recommend, the maximum excitation wavelength is practically limited to approximately 650 nm to prevent stray light from the excitation source reaching the detector. There is thus a relatively large section of the photosynthetically active spectrum where algal fluorescence dominates. A 'white' illumination source (Fig. 12a), for example, leads to a bias against cyanobacterial representation in community fluorescence. In contrast, a 'broad-green' light source (Fig. 12b) that excites predominantly accessory photosynthetic pigments yields near-equal representation of algal and cyanobacterial F v /F m . Our results show a relatively low correlation coefficient (R 2 = 0.33) of the community F v /F m with either group in the community, when we simulate the broad-green light source. Of course, many of the randomly mixed communities combine cultures exposed to widely different growth conditions and with very different F v /F m at a specific excitation-waveband pair, so that the community signal could never represent both subcommunities equally in these cases. The approach of simulating community fluorescence is, therefore, not to be used to interpret fluorometer performance beyond describing how well each group is represented in the community signal. In theory, the broad-green illumination band should predominantly excite accessory photosynthetic pigments, so that those phytoplankton groups that respond positively to the environmental conditions by producing accessory pigments, will dominate the result. This idea warrants further study, particularly in natural environments where such information may be desirable.
For multi-channel configurations, two narrow excitation bands located in the blue and orange-to-red constitute the minimum required combination to resolve some degree of subcommunity variable fluorescence information. Algal variable fluorescence is obtained with high accuracy from the blue channel. The extent to which orange excitation subsequently yields a different F v /F m will give some indication of the variable fluorescence of cyanobacteria in the community. This result is not unambiguous, because equal F v /F m from both blue and orange-excited fluorescence can be interpreted as equal F v /F m in algae and cyanobacteria but also as the absence of fluorescence from cyanobacteria. To differentiate the two cases, the ratio of F 0 intensities of blue versus orange excitation can be used to reveal whether cyanobacteria form a significant part of the community, because the presence of PBS pigment will certainly lead to a markedly higher orange-excited F 0 (results not shown). Of course, this suggested approach is similar to previous attempts to separate phytoplankton groups based on fluorescence excitation spectra (Millie et al. 2002;Beutler et al. 2002;Beutler et al. 2004;Parésys et al. 2005;Gaevsky et al. 2005;Seppälä and Olli 2008).
The small number of algal and cyanobacterial species used in our experiments, despite being grown in conditions to allow for a wide range in F v /F m , limits the applicability of our results. Fluorescence emission profiles of the major algae groups are relatively similar because the main source of fluorescence is always Chla located in PSII. The excitation spectrum, on the other hand, is dependent on the accessory photosynthetic pigments present. The choice of a single chlorophyte and diatom, representing red absorption by Chlorophylls b and c, is therefore still a realistic representation of many natural communities where algae and cyanobacteria co-exist. It does, however, not cover natural communities extensively. We may consider the case of phycobilin-producing rhodophytes and cryptophytes, as well as cryptophyte-ingesting ciliates (Gustafson et al. 2000) in further studies. The fluorescence excitationemission matrices of rhodophytes are similar to those of the cyanobacteria used here, although planktonic rhodophytes are generally few in environments where cyanobacteria are abundant. We hypothesize that the solutions for instrument design proposed here apply to these algae in the same manner as for the cyanobacteria described here. In contrast, the presence of phycoerythrin in cryptophytes and some dinoflagellates leads to a broader excitation domain in the algal groups. The presence of these 'special' algal groups in a natural sample will hamper efforts to decompose multi-channel fluorescence measurements into the contributions by individual groups (but see Seppälä and Olli 2008), even though it should not markedly change our definition of optimal excitation-emission bands to yield results that are most representative of the whole phytoplankton community.
The PBS pigments produced by strains in this study absorb yellow-to-red light as is common to freshwater and coastal species. The presence of oceanic species with forms of phycoerythrin absorbing down to 495 nm (Lantoine and Neveux 1997;Subramaniam et al. 1999;Neveux et al. 2006) would reduce the specificity of the blue-excited fluorescence signals to the algal part of the community, but we remain confident that the inclusion of an orange-to-red excitation band markedly increases sensitivity to the cyanobacteria present. Even with short-wavelength sensitive forms of phycoerythrin present, it is likely that the cyanobacteria will not be equally represented when using a narrow blue light source, which warrants further study.
To our knowledge, the present work constitutes the first effort to relate phytoplankton community variable fluorescence to the contributions from algal and cyanobacterial subpopulations over a wide domain of the spectral excitation-emission matrix. In order to collect this information with a standard, mid-range spectrofluorometer, some allowances have had to be made. We may question whether our analysis, based on dark adapted cells, manipulated in their growth environment to yield a range of F v /F m , are representative of results that would be obtained when using actinic light to manipulate F v 0 /F m 0 . We do believe that transient physiological change (i.e. state transitions) observed under (increasing) illumination can contribute to changes in the observed cyanobacterial influence on community variable fluorescence. At the same time, we assume that these changes are not likely to be of such magnitude that they would change our definition of the optimal fluorometer configuration. It would be most useful to see repeat experiments that focus on measuring F v 0 /F m 0 under varying actinic light intensities. A quantum-corrected FRRF or PAM instrument operating with multiple excitation bands would be an excellent platform for such investigations, simultaneously eliminating the need to use DCMU to induce F m .
In conclusion, we observe that microscope-based active fluorescence measurements, flow-cytometry, remote laser stimulated fluorescence and FRRF are examples of emerging methods in oceanography where phytoplankton fluorescence can shed more light on community composition and photosynthetic capacity at the subcommunity level. We foresee that the use of variable fluorescence techniques will gain increasing importance in environmental monitoring as a complementary method to carbon fixation measurements. It is therefore of prime importance to develop instruments and data interpretation techniques that are not biased against any of the major phytoplankton groups, particularly in environments where the physical environment is heterogeneous in time or space, and come to favour one functional group over another. The results presented in this paper will hopefully lead to a standardized and better understood variable fluorescence meter that will support studies of photosynthesis in optically complex environments.