Sarcoma-Virus-Related RNA Sequences in Normal Rat Cells

Tsuchida, Nobuo; Gilden, Raymond V.; Hatanaka, Masakazu

doi:10.1073/pnas.71.11.4503

Cited by 69 publications

(49 citation statements)

References 24 publications

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“…Equally strong cytoplasmic immunofluorescence appeared in cells 12 hr after exposure to 0.1 mM BrdU (Table 2). DISCUSSION Although it has been shown repeatedly that information for endogenous type C virus is present in normal rat cells (1,12,13), the mechanism(s) by which BrdU elicits virus synthesis is unclear. At optimal virogenic BrdU concentrations (0.1 mM), [3H]BrdU is incorporated uniformly into nuclear DNA sequences (2,3,14), whereas [3H]BrdU at suboptimal concentrations (0.1 ,uM) is nonrandomly distributed as determined by DNA-DNA reassociation techniques (2,3).…”

Section: Methodsmentioning

confidence: 99%

Distribution and virogenic effects of 5-bromodeoxyuridine in synchronized rat embryo cells.

Schwartz¹,

Panem²,

Kirsten³

1975

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

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Rat embryo cell cultures were synchronized by a double thymidine block. The DNA replication phase (S) was divided into an early, middle, and late period. Cell cultures in the early, middle, or late S phase were pulsed with 0.1 JM 5-bromo[3H]deoxyuridine (BrdU) or equimolar [3HldT. DNA The thymidine analog 5-bromodeoxyuridine (BrdU) induces the synthesis of a latent type C virus in secondary cultures of normal rat embryo cells (1). Release of type C particles into the culture fluids was first detected 2 days after BrdU removal, peaked 8-10 days later, and disappeared 14-16 days after removal of the analog. Density gradient centrifugation and DNA -DNA reassociation experiments revealed extensive and uniform base substitutions throughout the DNA sequences of rat embryo cells at the optimal virogenic BrdU dose (0.1 mM) (2). However, [3H] (2,3). The specific activity of each DNA sample was determined. Aliquots of radiolabeled DNA were centrifuged to equilibrium in gradients of neutral CsCl (2, 3). Gradient fractions were assayed for radioactivity, absorbance, and refractive index as described (2, 3).Renaturation Kinetics. Each DNA sample was made 0.40 M in sodium phosphate buffer, pH 6.8, and 3 mM in EDTA (2,3,7,8). The initial A260 of the reaction mixture was determined, and the sample was heat sealed in 5 ml glass ampoules and immersed completely in boiling water at 1000 for 10-15 min (2, 3, 7). After thermal denaturation, each ampoule was transferred to a 680 water bath and incubated until the product of initial DNA concentration (mol of 1829 Abbreviations: S, DNA replication phase of cell cycle; p30, group-specific antigen of Friend leukemia virus; BrdU, 5-bromodeoxyuridine; Cot, initial DNA concentration time.

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Section: Methodsmentioning

confidence: 99%

Distribution and virogenic effects of 5-bromodeoxyuridine in synchronized rat embryo cells.

Schwartz¹,

Panem²,

Kirsten³

1975

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

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“…Although similar in principle to that of other transforming retroviruses, the genetic organization of Ha-MuSV is more complex insofar as its 5.4-kilobase (kb) RNA genome is composed ofthree, rather than two, sets of sequences (8)(9)(10): (i) 0.1 kb at the 5' end and 0.9 kb at the 3' end, derived from the helper-independent virus Moloney murine leukemia virus; (ii) 3.5 kb sequences-highly homologous to a family of greatly reiterated rat genes, which are retroviral-like sequences expressed in many rat cellssometimes referred to as 30S sequences on the basis of the sedimentation coefficient of their RNA transcriptional product (28,29); and (iii) 1.0 kb of src sequences, completely bracketed by 30S sequences, that are required for transformation, encode the transformation-specific p21 protein, and originate from rat cellular sequences, which are highly conserved evolutionarily (10). As an initial step for investigating rat sarc sequences related to Ha-MuSV, we had defined a viral src probe from this latter set of sequences (10).…”

Section: Methodsmentioning

confidence: 99%

Analysis of two divergent rat genomic clones homologous to the transforming gene of Harvey murine sarcoma virus.

DeFeo¹,

Gonda²,

Young³

et al. 1981

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

270

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Harvey murine sarcoma virus (Ha-MuSV) is a mouse-rat recombinant retrovirus that encodes a protein designated p21, required for virally induced transformation. Using a radiolabeled DNA fragment from the p21 coding region, we have detected homologous DNA sequences in the normal DNA of rats and of several other vertebrate species. Moreover, many tested cells from these species contain low levels of a p21 protein that is highly related to viral 21. Now we report two independent fragments from normal rat DNA containing sequences (sarc) homologous to the Ha-MuSV transforming region that were cloned in the bacteriophage vector Charon 4A. Sarc sequences in the one fragment are completely colinear with the viral sequences and share apparently all restriction endonuclease sites. Sarc sequences in the second fragment have several sets of intervening sequences and lack some restriction endonuclease sites found in the viral transforming region. Despite the presence of these intervening sequences in the second sarc fragment, we have been able to ligate this sarc fragment to the long terminal repeat sequence of HaMuSV and to induce cellular transformation and high levels of p21 expression upon transfection of this DNA to NIH 3T3 mouse cells. These results suggest that elevated levels of p21, normally expressed at low levels in a variety of cells, can induce cellular transformation.Retroviruses can be grouped into two broad classes based upon their biological activities: the nontransforming leukemia or leukosis viruses and the transforming sarcoma or acute leukemia viruses (1). The molecular biology of the transforming viruses, such as Rous sarcoma virus, Moloney murine sarcoma virus (Mo-MuSV), Abelson murine leukemia virus, and Harvey murine sarcoma virus (Ha-MuSV), has been of special interest because viruses ofthis class enable cellular transformation related to a defined genetic sequence and its gene product(s) to be studied in great detail and under a high degree ofexperimental control. Accordingly, the genetic origin and transforming proteins of these viruses have come under close scrutiny (2-10).Our laboratory has been investigating the molecular biology of Ha-MuSV, a replication-defective retrovirus derived after injection of a mouse leukemia virus into a rat (11). Similar to sequences in the above-mentioned viruses, the Ha-MuSV src gene sequences are derived from (rat) cellular unique sequences (10). These viral src sequences encode the transformation-specific p21 protein (12, 13) and the p21 biochemical activities, which specifically use guanine nucleotides (14,15). Consistent with the conserved nature of these sequences is the expression ofa related, but distinguishable p21 sarc protein in normal cells from a wide variety of species (16).In order to understand better any differences in the structure, biology, and regulation of expression between the viral p21 src and the related cellular p21 sarc protein, we have initiated studies into the structure and function of rat sarc genes. In this report, we describ...

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“…The donor splice sequence has been altered in the Ha-MSV genome and apparently no longer functions (25). The two sequences abruptly diverge at this point, and the remaining 210 bp included in the Ha-MSV element are related to rat VL30 sequences (13,52 If the lack of enhancer activity was responsible for the block in viral expression in infected EC cells, then the relatively high frequency of G418 resistance obtained after pMLV.WT transfection (Table 1) as compared with FVXMneo infection (1 to 10 G418-resistant colonies per 106 infected cells) was surprising. This is especially true if one considers that viral infection is reportedly a much more efficient means of introducing exogenous genetic material (7).…”

mentioning

confidence: 99%

Proviral sequences that restrict retroviral expression in mouse embryonal carcinoma cells.

Loh¹,

Sievert²,

Scott³

1987

Mol. Cell. Biol.

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Embryonal carcinoma (EC) cells are nonpermissive for retrovirus replication. Restriction of retroviral expression in EC cells was studied by using DNA transfection techniques. To investigate the activity of the Moloney murine leukemia virus (M-MuLV) enhancer and promoter sequences, the M-MuLV long terminal repeat and the defined long terminal repeat deletions were linked to neo structural gene sequences that encode resistance to the neomycin analog G418. Transient expression data and drug resistance frequencies support the findings that the M-MuLV enhancer is not active in EC cells but that promoter sequences are functional. In addition, a proviral DNA fragment that encodes the leader RNA sequence of a M-MuLV recombinant retrovirus was found to restrict expression specifically in EC cells. Deletion analysis of the leader fragment localized the inhibitory sequences to a region that spans the M-MuLV tRNA primer binding site. It is not known whether restriction occurs at a transcriptional or posttranscriptional level, but steady-state RNA levels in transient expression assays were significantly reduced.

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Sarcoma-Virus-Related RNA Sequences in Normal Rat Cells

Cited by 69 publications

References 24 publications

Distribution and virogenic effects of 5-bromodeoxyuridine in synchronized rat embryo cells.

Distribution and virogenic effects of 5-bromodeoxyuridine in synchronized rat embryo cells.

Analysis of two divergent rat genomic clones homologous to the transforming gene of Harvey murine sarcoma virus.

Proviral sequences that restrict retroviral expression in mouse embryonal carcinoma cells.

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