Deborah R. Marino scite author profile

During early development, rat cardiac muscle cells actively proliferate. Shortly after birth, division of cardiac muscle cells ceases, whereas DNA synthesis continues for approximately 2 weeks at a progressively diminishing rate. Little DNA synthesis or cell division occurs in adult cardiocytes. Thus, developing cardiac muscle cells are an ideal system in which to examine the expression of cell cycle-regulated genes during development. We chose to examine proliferating cell nuclear antigen (PCNA), a gene expressed at the G1/S phase boundary of the cell cycle. Northern blots of RNA from cardiac muscle cells from 18-day-old rat fetuses and from day 0, 5, and 14 neonatal as well as adult rat hearts revealed that the PCNA mRNA was found in cardiac muscle cells from all ages. However, because it was possible that this was a result of fibroblast PCNA gene expression, we used reverse transcription followed by polymerase chain reaction to see if it was possible to detect the message for PCNA in cardiac muscle cells from all ages. Because of the great sensitivity of this technique, RNA was recovered from 25 isolated adult cardiac muscle cells. Polymerase chain reaction amplification products for PCNA produced from the RNA isolated from these cells conclusively demonstrated that mRNA for this gene, which normally is associated with proliferating cells, is expressed in adult cardiac muscle cells that no longer divide. Furthermore, Western blot analysis demonstrated that the PCNA protein was found only in embryonic and neonatal cells and not in adult rat cardiac muscle cells. Therefore, it might be inferred from these data that PCNA might be regulated at the posttranscriptional level in adult cardiac muscle cells.

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Relative sensitivity of the endogenous hprt gene and lacl transgene in ENU‐treated big blue™ B6C3F1 mice

Skopek

Kort

Marino

1995

Environ and Mol Mutagen

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Three-week-old Big Blue (BB) B6C3F1 mice were given a single i.p. injection of ENU. Three weeks later, splenic T cells were isolated from each animal by ficoll gradient centrifugation and divided into two samples. One sample was cultured to measure hprt- mutation and the other was used to extract DNA for lacI- analysis. T cells from BB mice exposed to 0, 4.5, 13.5, and 40 mg ENU/kg (9 or 10 animals per group) displayed dose-related increases in the frequency of both hprt- and lacI- mutations. Within each treatment group, the ENU-induced mutation frequency (average observed mutation frequency minus average control frequency) was remarkably similar at the two loci. This suggests that treatments that increase mutation frequency at the endogenous hprt gene also produce similar incremental increases at the BB lacI transgene. However, because of the ten-fold higher spontaneous mutation rate at lacI, the fold-increase over background produced by ENU at this locus was significantly less than the fold-increase produced at hprt. For example, the 4.5 mg ENU/kg treatment produced a 5.2-fold increase above background at hprt (P = 0.001), whereas only a 1.5-fold increase was produced at lacI (P = 0.140). Consequently, mutagenic insults that produce up to a fivefold increase in mutation frequency at an endogenous locus may be difficult to detect at the lacI transgene. Finally, the ENU-induced response at hprt in BB mice was identical to that in generic B6C3F1 mice, suggesting that there are no inherent differences between transgenic and normal mice in their response to this mutagenic agent.

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Caffeine Inhibition of Ochratoxin A Production

Buchanan

Tice

Marino

1982

Journal of Food Science

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The effect of caffeine and theobromine on growth and ochratoxin A production by AspergiZZus ochraceus was determined using microbiological medium. Caffeine produced a small decrease in growth, while reducing ochratoxin production as much as 98%. Theobromine had relatively little effect on growth or ochratoxin production. Screening of caffeine for its effect on the growth of a number of Aspergillus and Penicillium species indicated that caffeine may have biological activity against a variety of mycotoxigemc molds.Penicillium roqueforti M251 were also used to study the effect of caffeine on growth. The latter three species were obtained from the culture collection of the Dept. Food Science, Univ. of Georgia. Stock cultures w;re maintained on potato dextrose agar (D&o) slants stored at 4 C. Spore suspensions were prepared as previously described (Buchanan and Ayres, 1976), and diluted to lo6 conidia/ml.

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Pullulans produced by strains of Cryphonectria parasitica—I. Production and characterisation of the exopolysaccharides

Forabosco

Bruno

Sparapano

et al. 2006

Carbohydrate Polymers

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Deborah R. Marino

Proliferating cell nuclear antigen in developing and adult rat cardiac muscle cells.

Relative sensitivity of the endogenous hprt gene and lacl transgene in ENU‐treated big blue™ B6C3F1 mice

Caffeine Inhibition of Ochratoxin A Production

Pullulans produced by strains of Cryphonectria parasitica—I. Production and characterisation of the exopolysaccharides

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