Binding of anti-nucleoside antibodies reveals different classes of DNA in the chromosomes of the kangaroo rat ( Dipodomys ordii)

Abstract

Summary The binding of highly purified anti-nucleoside antibodies to fixed metaphase chromosomes of the kangaroo rat ( Dipodomys ordii ) revealed the presence of different classes of DNA in different regions of the chromosomes. To permit antibody binding, the chromosomal DNA was first made single-stranded by either ultraviolet irradiation, which denatures some classes of AT-rich DNA, or photo-oxidation, which denatures GC-rich DNA. The antibody binding patterns obtained matched the location of the different classes of satellite DNA in kangaroo rat chromosomes. After either denaturation method, anti-5-methylcytidine (anti-M) bound intensely only to the centromeric heterochromatic regions which are known to contain the GC rich, highly methylated HS- β satellite DNA of this species. The basic repeating unit of the HS- β sequence is 5′-ACACAGCGGG-3′ 3′-TGTGTCGCCC-5′ [4]. The binding of anti-M after UV irradiation is permitted by the production of pyrmidine (CC and TC) dimers in the right-hand portion of this repeating sequence, supporting the idea that the 5-methylcytosine residues are in this portion. After photo-oxidation, anti-cytidine (anti-C) and anti-adenosine (anti-A) also showed intense binding to the centromeric heterochromatin. In addition, these antibodies showed moderately intense binding to non-centromeric heterochromatic regions, which contain the relatively GC-rich HS- α and MS satellite DNAs. After UV irradiation, anti-A binding produced a banding pattern identical to the quinacrine (Q-band) pattern, with bright chromosome arms and very dull centromeric heterochromatic regions, while anti-C showed moderate binding in the centromeric regions and fairly even but weak binding elsewhere. The results have clarified the way in which anti-nucleoside antibodies react with chromosomal DNA. The reactivity of anti-A, anti-C and anti-M with the partially denatured HS- β satellite DNA supports the idea that antibody binding requires denaturation of a sequence perhaps no more than 5 base pairs long. In addition, it appears that it is not necessary to have more than one identical base in a row to permit antibody binding.