Analysis of Long Pyrimidine Polynucleotides in HeLa Cell Nuclear DNA: Absence of Polydeoxythymidylate

Birnboim, H.C.; Mitchel, R. E. J.; Straus, Neil A.

doi:10.1073/pnas.70.8.2189

Cited by 28 publications

(14 citation statements)

References 18 publications

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“…RNase digestion (pancreatic RNase cuts at C and U residues, while T1 RNase cuts at G) of this mRNA preparation revealed a resistant fraction presumed to be poly(A) (Lim and Canellakis 1970;Edmonds et al 1971;Adesnik et al 1972;Mendecki et al 1972;Birnboim et al 1973). Since long poly(A) tracts were not thought to be DNA-templated (Birnboim et al 1973;Jelinek et al 1973), a poly(A) polymerase was sought and found that was subsequently shown to be responsible for poly(A) tail formation on mRNA (Winters and Edmonds 1973a,b). The function of mRNA poly(A) could only be guessed at in these initial studies.…”

Section: Polyadenylation Signals and 39 Noncoding Rna (Ncrna) Sequencesmentioning

confidence: 94%

Ending the message: poly(A) signals then and now

Proudfoot¹

2011

Genes Dev.

528

486

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Polyadenylation [poly(A)] signals (PAS) are a defining feature of eukaryotic protein-coding genes. The central sequence motif AAUAAA was identified in the mid1970s and subsequently shown to require flanking, auxiliary elements for both 39-end cleavage and polyadenylation of premessenger RNA (pre-mRNA) as well as to promote downstream transcriptional termination. More recent genomic analysis has established the generality of the PAS for eukaryotic mRNA. Evidence for the mechanism of mRNA 39-end formation is outlined, as is the way this RNA processing reaction communicates with RNA polymerase II to terminate transcription. The widespread phenomenon of alternative poly(A) site usage and how this interrelates with pre-mRNA splicing is then reviewed. This shows that gene expression can be drastically affected by how the message is ended. A central theme of this review is that while genomic analysis provides generality for the importance of PAS selection, detailed mechanistic understanding still requires the direct analysis of specific genes by genetic and biochemical approaches.

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Section: Polyadenylation Signals and 39 Noncoding Rna (Ncrna) Sequencesmentioning

confidence: 94%

Ending the message: poly(A) signals then and now

Proudfoot¹

2011

Genes Dev.

528

486

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“…Since pyrimidine nucleotides are quite stable to this treatment they appear as nucleotides and a series of pyrimidine-containing oligonucleotides (1). When HeLa (human) DNA was degraded in this way, unexpectedly long pyrimidine tracts were found, in addition to the usual products of digestion (2). Both the size and number of these tracts differed greatly from that predicted assuming a random distribution of pyrimidines.…”

mentioning

confidence: 91%

“…Ninety percent formic acid (1.5 ml) -2.7% diphenylamine was added and the mixture was incubated for 18-20 hr at 300 in a darkened, Teflon-stoppered tube. Formic acid and diphenylamine were removed by a slight modification of our previous procedure (2). One milliliter of solution containing 10 M urea, 1 M sodium acetate, and 100 lig of tRNA was added to the hydrolysis mixture and it was extracted three times with 5 ml of diethyl ether.…”

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confidence: 99%

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Long Pyrimidine Tracts of L-Cell DNA: Localization to Repeated DNA

Straus

Birnboim

1974

Proc. Natl. Acad. Sci. U.S.A.

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Like HeLa DNA, L-cell DNA contains a significant number of unexpectedly long pyrimidine tracts. 1.3% of the thymidine residues of L-cell DNA are found in these long polypyrimidine tracts. Analysis of L-cell DNA fractions with different rates of reassociation indicates that polypyrimidine tracts are associated with "repeated" DNA. Longer pyrimidine tracts appear to have a higher repetition frequency than.shorter tracts, and some may be repeated as many as 5 X 104 times in L-cell DNA.Limited treatment of DNA with acid results in the release of purine bases and the breakage of the phosphodiester backbone. Since pyrimidine nucleotides are quite stable to this treatment they appear as nucleotides and a series of pyrimidine-containing oligonucleotides (1). When HeLa (human) DNA was degraded in this way, unexpectedly long pyrimidine tracts were found, in addition to the usual products of digestion (2). Both the size and number of these tracts differed greatly from that predicted assuming a random distribution of pyrimidines. Their unusual nature led us to examine DNA from a variety of eukaryotes, and similar polydeoxynucleotides were detected in several samples (Birnboim & Straus, manuscript in preparation). In particular, mouse L-cell DNA was found to contain more of these sequences than did other DNA's, and it was therefore chosen for further study. In the present report, we have utilized hydioxyapatite chromatography to fractionate L-cell DNA into "unique" and "repeated" sequences and have shown that long pyrimidine tracts are primarily localized in "repeated" DNA. min. This mixture was centrifuged at 3000 X g for 10 min and the aqueous phase was added to a column (2.54-cm diameter) containing 2 g of hydroxyapatite (HTP, Bio-Rad Laboratories). The hydroxyapatite was washed with the 8 M urea-PB solution until the 3H cpm/ml eluting from the column dropped to 1000 cpm/mi, and then with 0.014 M PB until the index of refraction of the effluent equaled that of the eluant.[8H]DNA was eluted with 0.

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“…There is evidence that these poly(A) sequences are not encoded in DNA, but are added post-transcriptionally: (a) cordycepin blocks synthesis of poly(A) and appearance of mRNA into the cytoplasm, but does not inhibit synthesis of HnRNA (5,7,8,11,12); (b) the number and size of poly(dT) sequences in mammalian nuclear DNA has been determined by isolation of polypyrimidine sequences in DNA after depurination; these poly(dT) sequences could account for only a very small fraction of the poly(A)200 sequences in mRNA (13); and (c) adenovirus type-2 mRNA contains poly(A) sequences of 100-200 bases, yet adenovirus DNA contains no poly(dT) sequences of equivalent size detectable by RNA DNA hybridization (14).…”

mentioning

confidence: 99%

Transcription of Polydeoxythymidylate Sequences in the Genome of the Cellular Slime Mold, Dictyostelium discoideum

Jacobson

Firtel

Lodish

1974

Proc. Natl. Acad. Sci. U.S.A.

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Messenger RNA of the cellular slime mold, Dictyostelium discoideum, contains about equimolar amounts of two classes of poly (adenylic acid) [poly(A)]; one is about 25 nucleotides long and the second about 100 nucleotides long. At least half of the messenger RNA molecules contain one sequence each of poly(A)25 and poly(A)soo; both poly(A) sequences are located near the 3' end of messenger RNA, and the kinetics of their appearance on messenger RNA precursor indicates that poly(A)25 is added before poly(A)soo. Dictyostelium nuclear DNA contains 14,000-15,000 sequences of poly(dT)25 which could code for the smaller poly(A) residues. The poly(A),oo must be added post-transcriptionally. The poly(dT)25 sequences are interspersed throughout the genome and may well represent transcription termination regions.Messenger RNA of mammalian cells contains, at the 3' end, a sequence of poly(adenylic acid) [poly(A)] of about 200 bases (1-9). Twenty to 40% of the giant heterogeneous nuclear RNA (HnRNA) molecules found in these cells also contain a poly(A) sequence at their 3' end (6,8). Because the poly(A) in the HnRNA is present at the 3' end, it has been suggested that the region of the HnRNA molecule nearest the 3'-end poly(A) is the material precursor of mRNA (7, 9, 10).There is evidence that these poly(A) sequences are not encoded in DNA, but are added post-transcriptionally: (a) cordycepin blocks synthesis of poly(A) and appearance of mRNA into the cytoplasm, but does not inhibit synthesis of HnRNA (5,7,8,11,12); (b) the number and size of poly(dT) sequences in mammalian nuclear DNA has been determined by isolation of polypyrimidine sequences in DNA after depurination; these poly(dT) sequences could account for only a very small fraction of the poly(A)200 sequences in mRNA (13); and (c) adenovirus type-2 mRNA contains poly(A) sequences of 100-200 bases, yet adenovirus DNA contains no poly(dT) sequences of equivalent size detectable by RNA DNA hybridization (14).We previously showed that mRNA from Dictyostelium contains a poly(A) sequence of 40-150 nucleotides, with a mean size of 100 at the 3' end (15). We report here that mRNA also contains a sequence of poly (A) (15,16). Dictyostelium nuclei were isolated and utilized for cell-free RNA synthesis as described (17).Isolation of Poly(A). Either total RNA, or poly(A)-containing RNA purified by chromatography on poly(U)-Sepharose, was used. RNAs were digested at 370 for 30-60 min in 0.36 M Na+ by 10 units/ml of RNase T, and 5 ,ug/ml of RNase A. Sodium dodecyl sulfate (0.5%) and proteinase K (1 mg/ml) were added to terminate the reaction. After an additional incubation at 300, the mixture was extracted with phenol-chloroform and the poly(A) material was purified by adsorption to and elution from poly(U)-Sepharose or oligo-(dT)-cellulose (15,16). Finally the poly(A) was precipitated with ethanol, with Escherichia coli tRNA as carrier. The size and base composition of the poly(A) sequences were the same whether or not the poly(A)-containing RNA was first purified by chro...

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Analysis of Long Pyrimidine Polynucleotides in HeLa Cell Nuclear DNA: Absence of Polydeoxythymidylate

Cited by 28 publications

References 18 publications

Ending the message: poly(A) signals then and now

Ending the message: poly(A) signals then and now

Long Pyrimidine Tracts of L-Cell DNA: Localization to Repeated DNA

Transcription of Polydeoxythymidylate Sequences in the Genome of the Cellular Slime Mold, Dictyostelium discoideum

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