6533b86cfe1ef96bd12c8a90

RESEARCH PRODUCT

Chromosome Analysis and rDNA FISH in The Stag Beetle Dorcus Parallelipipedus L. (Coleoptera: Scarabaeoidea: Lucanidae)

Mario ZuninoMariastella ColombaRoberto Vitturi

subject

MaleSilver StainingStag beetleZoologyScarabaeoideaDNA RibosomalChromosomesGiemsa stainHeterochromatinNucleolus Organizer RegionGeneticsAnimalsRibosomal DNAIn Situ Hybridization FluorescenceGeneticsbiologyChromosomeGeneral MedicineDorcus parallelipipedusRibosomal RNAbiology.organism_classificationChromosome BandingColeopteraKaryotypingFemaleNucleolus organizer region

description

In the present work the chromosome complement (2n = 18; 8AA + XY) of the stag beetle Dorcus parallelipipedus L. (Scarabaeoidea: Lucanidae) is analyzed using conventional Giemsa staining, banding techniques and ribosomal fluorescent in situ hybridization (rDNA FISH). rDNA FISH remains the unique tool for providing a clear-cut identification of Nucleolar Organizer Regions (NORs) when conventional banding methods such as silver- and CMA3-staining proved to be inadequate. The dull, homogeneous CMA3 fluorescence of all chromosomes indicates the absence of markedly GC rich compartmentalized regions in D. parallelipipedus genome. Silver impregnation inadequacy in detecting NOR regions is to be sought in the unusual extensive silver stainability of heterochromatic material which, on the contrary of what stated for vertebrates, seems to be a common feature in Scarabaeoidea species.

yearjournalcountryeditionlanguage
2001-07-04Hereditas
https://doi.org/10.1111/j.1601-5223.2000.00249.x