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Revista de Biología Tropical

On-line version ISSN 0034-7744Print version ISSN 0034-7744

Rev. biol. trop vol.52  suppl.1 San José Sep. 2004

 

The use of pigment "fingerprints" in the study of harmful algal blooms

 

J. Bustillos-Guzmán1 , I. Gárate-Lizárraga2 , D. López-Cortés1 & F. Hernández-Sandoval1

1 Centro de Investigaciones Biológicas del Noroeste. POB 128, La Paz, Baja California Sur, México. Fax: +52 612 12 5 47 10; jose@cibnor.mx.

2 Departamento de Plancton y Ecología Marina, CICIMAR-IPN, POB 592, La Paz, Baja California Sur, México.

 

Recibido 31-X-2002. Corregido 11-VI-2003. Aceptado 11-XII-2003.

 

Abstract

Along the Mexican coast, harmful algae blooms (HAB) have become more frequent, and therefore, there is an urgent need to establish monitoring programs to avoid the undesired consequences of HAB in human and natural ecosystems. In this work, we analyzed the pigment signatures and the species composition from phytoplankton samples to evaluate the utility of the specific pigment "fingerprints" in HAB monitoring programs. Vertical profiles from a coastal lagoon and temporal samples of a red tide occurring in a shrimp-culture pond and in a coastal zone were taken into consideration. Between 76% and 84% of dinoflagellate and diatom cell density was explained by their specific signature variation, in both vertical and temporal samples. Only the variation of zeaxanthin and the cyanobacteria Anabaena sp. showed a poor relationship, probably from difficulties in counting other cyanobacteria present in the samples examined with the microscopic method. These results suggest that inclusion of pigment analysis in the study and monitoring programs dealing with harmful algae would be very useful.

Key words: HPLC, HAB, pigments, monitoring, dinoflagellates.

Palabras clave: HPLC, PAN, pigmentos, monitoreo, dinoflagelados.

 

 

Although the use of pigments in studies of distribution and abundance of phytoplankton in the oceans was suggested in the 1960s (Jeffrey 1961, 1968), its use was seriously limited because thin layer chromatography lacked instrumentation to get a better performance of the process. New developments in HPLC techniques permitted good separation and quantification of most of the algal pigments (Mantoura and Llewellyn 1983). At present, improvements in HPLC methods have allowed the separation of a wide array of pigment, including both polar chlorophyll (chl), c-type pigments (chl c1 , chl c2 , chl c3 ) and non-polar (chl a and b plus its DV forms, non-polar chl c), as well as carotenoids in a single run (Goericke and Repeta 1993, Vidussi et al. 1996, Zapata et al. 1998). Among the estimated phytoplankton species, about 7% (300 species) are known to produce red tides and of those, only 2% are actually harmful or toxic (Smayda 1997).

Dinoflagellates, diatoms, prymnesiophytes, and more recently, raphydophytes species are the main contributors to this list, and each of them has particular pigment "fingerprints" that, at the level group, can be identified (reviewed in Jeffrey and Vesk 1997). Further, HPLC methods with mathematical tools (Mackey et al. 1996) for interpreting data, have provided invaluable information about the variability of phytoplankton populations under changeable hydrographic conditions (Barlow et al. 1993, Claustre et al. 1994, Bustillos-Guzmán et al. 1995), and have permitted identification of "uncommon" phytoplanktonic groups (Bustillos-Guzmán et al. 2001).

Pigment signatures in the study of HABs have been very limited, particularly in monitoring programs (Yacobi et al. 1996, Gárate-Lizárraga et al. 2000, López-Cortés et al. 2003). Along the Mexican Pacific coast, dinoflagellates are the main group responsible for red tides (Cortés-Altamirano et al. 1996, Gárate-Lizárraga et al. 2001a). Other groups, such as diatoms, particularly the Pseudonitzschia complex (a DSP-producer), prymnesophytes, and chlorophytes also form blooms, but with less frequency (Hernández-Becerril 1998, Gárate-Lizárraga et al. 2001a). All of the above-mentioned bloom-forming species, have pigment signatures (Table 1) that could be useful in tracking and following them as they occur in nature. We illustrate the use of pigment signatures to follow the spatial and temporal distribution of potential HAB species and how these signatures could be related to the variation of cell density.

 

 

Materials and methods

Field Sampling

Case 1: vertical distribution

To obtain samples for pigment analysis of the phytoplankton community from Bahía Concepción, water was collected at 0, 8, 10, 20, 21, 22, 24, and 25 m depth with a van Dorn bottle. This bay is one of the largest on the west coast of the Gulf of California (located between the 26°33’ and 26°53’ N and 111°42’ and 112°56 W) with low human impact and well-known occurrences of HABs (Lechuga-Deveze and Morquecho-Escamilla 1998, Bustillos-Guzmán et al. 2000, Gárate-Lizárraga et al. 2001b).

Case 2a: temporal variation

An intense-brown bloom was observed in a shrimp-culture pond located in Bahía de La Paz, Gulf of California (24 o 10’ N and 110 o 18’ W). From this pond, daily surface samples were taken for taxonomic identification, cell-counting, and pigment analysis. Sampling started on August 21 th and stopped on September 15th 1998 when the causative organism of this bloom was scarce. The pond was fertilized, as part of the shrimp-culture cycle, every week with phosphates and nitrates during the sampling period, to stimulate algal productivity.

Case 2b: temporal variation

On September 15th 2000, several small red tide areas were found in La Ensenada de La Paz. Cochlodinium polykrikoides Margalef was the responsible dinoflagellate (Gárate-Lizárraga et al. 2000). From September 15th to 29th (until the algal bloom was no longer visible), samples were taken from the middle of the algal bloom. Number of daily samples varied, since conditions, mainly wind and tidal dynamics, and dinoflagellate migration behavior (Park et al. 2001), avoided the location of the red tide spots.

 

Laboratory Analysis

Pigment analysis

All water samples were ice cooled and kept in the dark for transportation to the laboratory (maximum of 1.5 hours). Water was GF/F filtered and the filters were extracted with 2 ml of 100% acetone in an ice bath, hand ground with a glass rod, and stored overnight at -40°C to fully extract. Extract was recovered after centrifugation (3 000 g for 5 min). The extract (200 µl) was mixed with 100 µl 0.5 N ammonium acetate and injected through a 100-µl loop into an HPLC system (Hewlett Packard series 1100) with a photodiode array detector (1.2 nm optical resolution). Pigments were separated and quantified by isocratic HPLC in a reverse-phase, as described in Vidussi et al. (1996). Mobile phase consisted of MeOH: 0.5 N aqueous ammonium acetate, 70:30% v/v (solvent A), and MeOH (solvent B), with a gradient (minute; percent of solvent A- percent of solvent B): 0;75-25, 1;50-50, 15;0-100, and 19;75-25. Quantification was based on the absorbance at 440 nm and the factor response (peak area / pigment concentration) value for each pigment, as described in Mantoura and Repeta (1997). Identification of the pigment marker for each group (Table 1) considered retention time, spectral characteristics, and chromatography with certified commercial standards (International Agency for 14 C determinations, Denmark). Samples for identification and cell-counting were fixed and preserved with lugol. Samples were analyzed in 5-ml settling chambers and observed with a phase contrast inverted microscope (Hasle 1978).

 

Results

Vertical variation

Fig. 1 shows a representative chromatogram for each example from this work. In Bahía Concepción, surface pigments were chlorophyll a, zeaxanthin, fucoxanthin, chlorophyll c1-2 , and minor quantities of fucoxanthin-like carotenoids and b -carotene (Fig. 1A). Below 20 m, a new series of pigments (peaks 11 to 16 and 20, Fig. 1B), characteristics of anoxygenic phototrophic bacteria (Bustillos-Guzmán et al. 2000) were present, together with peridinin and fucoxanthin. This vertical distribution of pigments shows that there exists a pigment subsurface maximum concentration between 20 and 25 m (Fig. 2). Maximum values are for peridinin and fucoxanthin (Fig. 2A, B). Above this maximum, zeaxanthin is the main pigment (Fig. 2C). Maximal values of peridinin and fucoxanthin were related to the dinoflagellates, Heterocapsa niei Morril et Loeblich (>130 000 cells/l) and Prorocentrum dentatum Stein (>6 000 cells/l) and the diatom Nitzschia longissima Smith (>3 000 cells/l). Cell density of dinoflagellates and diatoms was clearly related to their pigment signature variations (Fig. 3A, B). In the upper layer (<20 m), the chain forming cyanobacteria Anabaena sp. was conspicuous, however, no significant relationship with zeaxanthin was found (Fig. 3C).


 


 


Temporal variation

Pigments composition shows that phyto-plankton in these samples had peridinin, diadinoxanthin, and chlorophylls a and c2 (Fig. 4). This pigment profile corresponds to the typical pigments of dinoflagellates (Johansen et al. 1974, Jeffrey et al. 1975). The dinoflagellate responsible for this bloom was Scrippsiella sp. Small amounts of fucoxanthin and chlorophyll b were present because of benthic diatoms (Amphora spp.) and the prasinophyte Nephroselmis sp.


 
Temporal pigment variation shows that peridinin fluctuates between 8 and 50 µg peridinin/ l before and after the peak concentration (109 µg peridinin/l), on September 3rd (Fig. 5A). The higher concentration of fucoxanthin and chlorophyll b did not coincide with the peak peridinin concentration and was relatively low, compared with peridinin concentrations. Density of Scrippsiella sp. and peridinin were closely related (Fig. 5B).



C. polykrikoides blooms also showed typical pigment composition of dinoflagellates. In addition, small amounts of fucoxanthin and chlorophyll b indicated the presence of tychoplanktonic diatoms and small flagellates (Fig. 6). As stated earlier, small areas of C. polykrikoides were easily dispersed, so the number of daily samples was variable. Peridinin concentration reached values as high as 32 µg/l in one spot on September 20th (Fig. 7A). Cell density was also high on this date and reached more than 7 x 106 cells/l. Both C. polykrikoides density and peridinin changes were related (Fig. 7B).





Discussion

Our results clearly show that pigment signatures varied with cell density of the phytoplankton group that contains the marker and supports this approach to monitoring HAB. However, although significant, the relationships were not perfect and 76 to 84% of the variability in cell-density was explained by the variations of the pigments. Conversely, the relationship between zeaxanthin concentration and Anabaena sp. in the vertical pigment profile in Bahía Concepción was not significant. Variations in cell pigment content in phytoplankton depend on factors, such as light (Falkowski and LaRoche 1991, Johansen and Sakshaug 1993) and nutrient and species composition (Bustillos-Guzmán and Diogene 1998, Tang 1996). Natural samples, include a mix of populations in different physiological stages, and hence, pigment content. These variables reasonably explain less-than-perfect correlations of pigments and cell density. The poor relationship between Anabaena sp. cell density and zeaxanthin could be explained because cyanobacteria identification is difficult. Some do not form chains and are very small. It is possible that other cyanobacterial species were present in the Bahía Concepción samples, but the above-mentioned difficulties make clear identification unlikely. Therefore, by not considering these species, the lower accuracy of zeaxanthin for biomass estimates must be considered for non-dominant cyanobacteria.

Pigment utility in phytoplankton studies has been widely demonstrated and generated new knowledge in marine ecology (reviewed by Jeffrey et al. 1997). However, their use in monitoring programs (Yacobi et al. 1996), particularly in HAB events in México has been very limited. As far as we know, monitoring of HAB by using pigments, has been limited to Bahía Concepción, and the Gulf of California (Gárate-Lizárraga et al. 2001b, López-Cortés et al. 2003), although other programs, where traditional methods are used, are active (Cortés-Altamirano et al. 1996). In this bay, Gárate-Lizárraga et al. (2002a) have been able to track important densities of Gymnodinium catenatum and Alexandrium affine at the base of the nutricline by using the peridinin record. G. catenatum has been identified as the causative vector of human deaths in the Mazatlán area (Mee et al. 1986). Thus, even under conditions in which the HAB species would not have a "visible" signal, the monitoring of the pigment marker is useful. The need to include this approach in monitoring programs is highly encouraging from these results. As an example, a high temporal and spatial sample stations zone can be monitored firstly to track HAB pigment signatures. When concentrations of pigment markers of HAB species are recorded, efforts to address this zone for taxonomic and toxin analysis can be undertaken. The pigment signature approach to studying HAB presents advantages because it requires a short time for sample analysis (20- 25 minutes) and can be used to study HABs that require considerable time and effort to identify particular species, especially when its taxonomical characteristics are difficult to discern under light microscopy. Further, in the pigment signature approach, the highest levels of technical skills are not needed, as is the case of taxonomic studies.

 

Acknowledgments

The authors thank the National Council of Science and Technology (CONACyT) for financial and logistical support (grants 33684- V and 007PÑ-1297); F. Zapata-Vazquez for his assistance during fieldwork and I. Fogel for English language editing. This research was supported in part by CIBNOR Institutional Research Project AYCG-11 and AYCG3. IGL is COFAA, EDI, and CONACYT fellow (138138).

 

Resumen

A lo largo de las costas mexicanas, los florecimientos algales nocivos (FAN) se han vuelto cada vez mas frecuentes y por lo tanto, existe una necesidad urgente de establecer programas de monitoreo para evitar las consecuencias no deseadas por su desarrollo, sobre los ecosistemas naturales y el ser humano. En este trabajo, nosotros analizamos las huellas pigmentarias y la composición de especies de diversas muestras de fitoplancton para evaluar la utilidad que pueden representar estos pigmentos específicos o "huellas pigmentarias" en programas de monitoreo de florecimientos algales nocivos. Los perfiles verticales de muestras de fitoplancton de una laguna costera y muestras de mareas rojas que ocurrieron en un estanque de cultivo de camarón y en una laguna costera, fueron considerados en este estudio. Tanto en muestras verticales como en temporales, entre el 76% y 84% de la densidad celular de dinoflagelados y diatomeas fueron explicados por la variación de su huella específica, mientras que la variación de zeaxantina y la densidad de la cianobacteria Anabaena sp. mostró una relación pobre, la cual fue debida probablemente a la dificultad en el conteo que presenta este grupo al ser analizadas mediante un microscópico invertido. Estos resultados sugieren que la inclusión del análisis de las huellas pigmentarias en los programas del estudio y monitoreo de las algas nocivas sería de gran utilidad.

 

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