Summary
Techniques used for the transfer of novel genes into host plant genomes have created new possibilities for crop improvement. The implementation of transgenic crop species into agriculture has introduced the possibility of transgene escape into the environment via pollen dispersal. Although the movement of pollen is a critical step in transgene escape, there is currently no system to monitor transgenic pollen movement under field conditions. The development of an effective in vivo monitoring system suitable for use under field conditions is needed for research and commercial purposes so potential risks can be quantified and evaluated. This chapter describes the development of a model system using green fluorescent protein (GFP) expression in pollen as a marker to monitor pollen distribution patterns. A pollen specific promoter was used to express the GFP gene in tobacco (Nicotiana tabacum L.). GFP was visualized in pollen and growing pollen tubes using fluorescent microscopy. Furthermore, the goal of this research was to compare the dynamics of pollen movement with that of gene flow by using another method of whole plant expression of GFP (see Chapter 15) to estimate out-crossing frequencies by progeny analysis. Pollen movement and gene flow were quantified under field conditions. Pollen traps were collected and screened for presence of GFP-tagged pollen using fluorescence microscopy. Progeny from wild type plants were screened with a hand held ultraviolet light for detection of the GFP phenotype.
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References
Slatkin, M. (1985) Gene flow in natural populations. Annu. Rev. Ecol. Syst. 16, 393–430.
Slatkin, M. and Barton, N. H. (1989) A comparison of three indirect methods for estimating average levels of gene flow. Evolution 43, 1349–1368.
Ellstrand, N. C., Delvin, B., and Marshall, D. L. (1989) Gene flow by pollen into small populations: data from experimental and natural strands of wild radish. Proc. Natl. Acad. Sci. USA 86, 9044–9047.
Ellstrand, N. C. (1992) Gene flow among seed plant populations. New Forests 6, 241–256.
Friedman, S. T. and Adams, D. L. (1985) Estimation of gene flow into two seed orchards of loblolly pine (Pinus taeda L.). Theor. Appl. Genet. 69, 609–615.
Adams, W. T. and Birkes, D. S. (1990) Estimating mating patterns in for trees populations, in Biochemical Markers in the Population Genetics of Forest Trees, (Hattemer, H. H. and Fineschi, S. eds.), S.P.B. Academic Publishing, The Hague, The Netherlands, pp. 157–172.
Dow, B. D. and Ashley, M. V. (1998) High levels of gene flow in bur oak revealed by paternity analysis using microsatellites. J. Hered. 89, 62–70.
Stewart, C. N. Jr. (1996) Monitoring transgenic plants using in vivo markers. Nat. Biotech. 14, 682.
Leffel, S., Mabon, S. A., and Stewart, C. N. Jr. (1997) Application of green fluorescent protein in plants. BioTechniques 23, 912–918.
Harper, B. K., Mabon, S. A., Leffel, S. M., et al. (1999) Green fluorescent protein as a marker for expression of a second gene in transgenic plants. Nat. Biotech. 17, 1125–1129.
Halfhill, M. D., Warwick, S. I., Raymer, P. L., Millwood, R. J., and Weissinger, A. K. (2003) Gene flow from transgenic oilseed rape and crop x weed hybrids under field conditions. Environ. Bio. Res., in press.
Hudson, L. C., Chamberlain, D., and Stewart, C. N., Jr. (2001) GFP-tagged pollen to monitor pollen flow of transgenic plants. Mol. Ecol. Notes 1, 321–324.
Twell, D., Yamaguchi J., Wing, R. A., Ushiba, J., and McCormick, S. (1991) Promoter analysis of genes that are coordinately expressed during pollen development reveals pollen-specific enhancer sequences and shared regulatory elements. Genes Develop. 5, 496–507.
Wing, R. A., Yamaguchi J., Larabell S. K., Ursin, V. M., and McCormick S. (1989) Molecular and genetic characterization of two pollen expressed genes that have sequence similarity to pectate lyases of the plant pathogen Erwinia. Plant Mol. Biol. 14, 17–28.
Haseloff, J., Siemering, K. R., Prasher, D. C., and Hodge, S. (1997) Removal of a cryptic intron and subcellular localization of green fluorescent protein are required to mark transgenic Arabidopsis plants brightly. Proc. Natl. Acad. Sci. USA 94, 2122–2127.
Murashige, T. and Skoog, F. (1962) A revised medium for rapid growth and bioassays with tobacco tissue cultures. Physiol. Plant 15, 473–497.
Brewbaker, J. L. and Kwack, B.H. (1963) The essential role of calcium ion in pollen germination and tube growth. Am. J. Bot. 50, 589–865.
Saeglitz C., Pohl, M., and Bartsch, D. (2000) Monitoring gene escape from transgenic sugar beet using cytoplasmic male sterile bait plants. Mol. Ecol. 9, 2035–2040.
Horsch, R. B., Fry, J. E., Hoffman, N. L., Eichholts, D., Rogers, S. G., and Fraley R. T. (1985) A simple method for transferring genes into plants. Science 227, 1229–1231.
McCormick, S., Niedermeyer, J., Fry, J., Barnanson, A., Horsch, R., and Fraley, R. (1986) Leaf disc transformation of cultivated tomato (L. esculentum) using Agrobacterium tumefaciens. Plant Cell Rep. 5, 81–84.
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Hudson, L.C., Halfhill, M.D., Stewart, C.N. (2005). Transgene Dispersal Through Pollen. In: Peña, L. (eds) Transgenic Plants: Methods and Protocols. Methods in Molecular Biology™, vol 286. Humana Press. https://doi.org/10.1385/1-59259-827-7:365
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DOI: https://doi.org/10.1385/1-59259-827-7:365
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