Marking cell layers with spectinomycin provides a new tool for monitoring cell fate during leaf development

doi:10.1093/jexbot/51.351.1713

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Journal of Experimental Botany, Vol. 51, No. 351, pp. 1713-1720, October 2000
© 2000 Oxford University Press

Original Papers

Marking cell layers with spectinomycin provides a new tool for monitoring cell fate during leaf development

K. Pyke¹^,3, M.K. Zubko² and A. Day²

¹ School of Biological Sciences, Royal Holloway, University of London, Egham, Surrey TW20 0EX, UK
² School of Biological Sciences, Manchester University, 3.614 Stopford Building, Oxford Road, Manchester M13 9PT, UK

Spectinomycin, an inhibitor of plastid protein synthesis, canbe used to mark specific cell layers in the shoot meristem ofBrassica napus. Pale yellow-green (YG) plants resulting fromspectinomycin-treatment can be propagated indefinitely in vitro.Microscopic examination showed that YG-plants result from inactivationof plastids in the L2 and L3 layers and are composed of a palegreen epidermis covering a white mesophyll layer. Epidermalcells of YG and normal green plants are similar and contain10–20 small pale green plastids. YG plants are equivalentto periclinal chimeras with the important distinction that thereis no genotypic difference between the white and green celllayers. Periclinal divisions of epidermal cells take place atall stages of leaf development to produce invaginations of greenmesophyll located in sectors of widely varying sizes. A periclinaldivision rate of 1 in 3000–4000 anticlinal divisions forthe adaxial epidermis, was 2–3-fold higher than that estimatedfor the abaxial epidermis. Analysis of white and green mesophyllshowed that chloroplasts are essential for palisade cell differentiationand this requirement is cell-autonomous. Stable marking of celllineages with spectinomycin is simple, rapid and reveals therequirement for functional plastids in cellular differentiation.

Key words: Brassica, cell lineage, epidermis, leaf development, spectinomycin.

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