Literature DB >> 17951594

Cytochemistry and C-values: the less-well-known world of nuclear DNA amounts.

J Greilhuber1.   

Abstract

BACKGROUND: In the plant sciences there are two widely applied technologies for measuring nuclear DNA content: Feulgen absorbance cytophotometry and flow cytometry (FCM). While FCM is, with good reasons, increasingly popular among plant scientists, absorbance-cytophotometric techniques lose ground. This results in a narrowing of the methodological repertoire, which is neither desirable nor beneficial. Both approaches have their advantages, but static cytophotometry seems to pose more instrumental difficulties and material-based problems than FCM, so that Feulgen-based data in the literature are often less reliable than one would expect. SCOPE: The purpose of this article is to present a selective overview of the field of nuclear DNA content measurement, and C-values in particular, with a focus on the technical difficulties imposed by the characteristics of the biological material and with some comments on the photometrical aspects of the work. For over 20 years it has been known that plant polyphenols cause problems in Feulgen DNA cytophotometry, since they act as major staining inhibitors leading to unreliable results. However, little information is available about the chemical classes of plant metabolites capable of DNA staining interference and the mechanisms of their inhibition. Plant slimes are another source of concern.
CONCLUSIONS: In FCM research to uncover the effects of secondary metabolites on measurement results has begun only recently. In particular, the analysis of intraspecific genome size variation demands a stringent methodology which accounts for inhibitors. FCM tests for inhibitory effects of endogenous metabolites should become obligatory. The use of dry seeds for harvesting embryo and endosperm nuclei for FCM and Feulgen densitometry may often provide a means of circumventing staining inhibitors. The importance of internal standardization is highlighted. Our goal is a better understanding of phytochemical/cytochemical interactions in plant DNA photometry for the benefit of an ever-growing list of plant genome sizes.

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Year:  2007        PMID: 17951594      PMCID: PMC2710206          DOI: 10.1093/aob/mcm250

Source DB:  PubMed          Journal:  Ann Bot        ISSN: 0305-7364            Impact factor:   4.357


  39 in total

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3.  Absorption microphotometry of irregular-shaped objects.

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Journal:  Cytometry A       Date:  2006-04       Impact factor: 4.355

5.  Some characteristics of the cold hydrolysis technique for staining plant tissues by the feulgen reaction.

Authors:  D P Fox
Journal:  J Histochem Cytochem       Date:  1969-04       Impact factor: 2.479

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Journal:  Ann Bot       Date:  2006-07-04       Impact factor: 4.357

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Journal:  Ann Bot       Date:  2006-07-04       Impact factor: 4.357

Review 8.  Psoralens and their application to the study of some molecular biological processes.

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10.  DNA density in mitotic and meiotic metaphase chromosomes of plants and animals.

Authors:  M D Bennett; J S Heslop-Harrison; J B Smith; J P Ward
Journal:  J Cell Sci       Date:  1983-09       Impact factor: 5.285

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  15 in total

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5.  Effects of phenylcarboxylic acids on mitosis, endoreduplication and expression of cell cycle-related genes in roots of cucumber (Cucumis sativus L.).

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6.  Comparative cytogenetic analysis of the genomes of the model grass Brachypodium distachyon and its close relatives.

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Journal:  Ann Bot       Date:  2009-07-25       Impact factor: 4.357

7.  Evolution of genome size in Carex (Cyperaceae) in relation to chromosome number and genomic base composition.

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8.  Cardiomyogenesis in the aging and failing human heart.

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Review 9.  Genome size diversity in orchids: consequences and evolution.

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