Whole-Cell Immunolocalization of Nitrogenase in Marine Diazotrophic Cyanobacteria, Trichodesmium spp.

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Applied and Environmental Microbiology, August 1998, p. 3052-3058, Vol. 64, No. 8
0099-2240/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Whole-Cell Immunolocalization of Nitrogenase in Marine Diazotrophic Cyanobacteria, Trichodesmium spp.

Senjie Lin,¹^,^* Sheri Henze,¹ Pernilla Lundgren,² Birgitta Bergman,² and Edward J. Carpenter¹

Marine Sciences Research Center, State University of New York, Stony Brook, New York 11794,¹ and Department of Botany, Stockholm University, S-10691 Stockholm, Sweden²

Received 23 March 1998/Accepted 29 May 1998

The mechanism by which planktonic marine cyanobacteria of the genus Trichodesmium fix N₂ aerobically during photosynthesiswithout heterocysts is unknown. As an aid in understanding howthese species protect nitrogenase, we have developed an immunofluorescencetechnique coupled to light microscopy (IF-LM) with which intactcyanobacteria can be immunolabeled and the distribution patternsof nitrogenase and other proteins can be described and semiquantified.Chilled ethanol was used to fix the cells, which were subsequentlymade permeable to antibodies by using dimethyl sulfoxide. Useof this technique demonstrated that about 3 to 20 cells (mean± standard deviation, 9 ± 4) consecutively arranged in a Trichodesmiumtrichome were labeled with the nitrogenase antibody. The nitrogenase-containingcells were distributed more frequently around the center of thetrichome and were rarely found at the ends. On average 15% ofover 300 randomly encountered cells examined contained nitrogenase.The percentage of nitrogenase-containing cells (nitrogenase index[NI]) in an exponential culture was higher early in the lightperiod than during the rest of the light-dark cycle, while thatfor a stationary culture was somewhat constant at a lower levelthroughout the light-dark cycle. The NI was not affected by treatmentof the cultures with the photosynthetic inhibitor dichloro 1,3'-dimethylurea or with low concentrations of ammonium (NH₄Cl). However,incubation of cultures with 0.5 µM NH₄Cl over 2 days reduced theNI. The IF technique combined with ¹⁴C autoradiography showed that the CO₂ fixation rate was lowerin nitrogenase-containing cells. The results of the present studysuggest that (i) the IF-LM technique may be a useful tool forin situ protein localization in cyanobacteria, (ii) cell differentiationoccurs in Trichodesmium and only a small fraction of cells ina colony have the potential to fix nitrogen, (iii) the photosyntheticactivity (CO₂ uptake) is reduced if not absent in N₂-fixing cells,and (iv) variation in the NI may be a modulator of nitrogen-fixingactivity.

^* Corresponding author. Mailing address: Marine Sciences Research Center, State University of New York, Stony Brook, NY 11794.Phone: (516) 632-8697. Fax: (516) 632-8820. E-mail: selin{at}ccmail.sunysb.edu.

Contribution no. 1115 of the Marine Sciences Research Center.

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