Your search keyword '"Uccelli R"' showing total 5 results

1. Effects of heat on mouse spermatogenesis monitored by flow cytometry.

Author

De Vita R, Calugi A, Chiarantano C, Forte D, Mauro F, and Uccelli R

Subjects

Animals, DNA analysis, Flow Cytometry, Male, Mice, Organ Size, Testis anatomy & histology, Hot Temperature adverse effects, Spermatogenesis

Abstract

The effects of heat on mouse spermatogenesis have been determined using both testis weight and flow cytometrically determined DNA content distribution as experimental end-points. Temperatures of 38-42 degrees C and exposure times of 20-60 min have been tested. The results concerning the testis weight substantially confirm those reported by other authors (Hand et al. 1979). The measurement of DNA content distributions shows a relatively higher depletion, 14 days after treatment, of the cytometric compartment containing elongated spermatids in respect to that containing round spermatids. The analysis of the cytotoxic effects, monitored 14 vs. 28 days after treatment, as a function of the exposure time at a given temperature, or of the temperature for a fixed exposure time, indicates that, in the course of spermatogenesis, late spermatocytes are more sensitive to heat than differentiated spermatogonia. Following the approach based on flow cytometry, the effect of exposures as low as 20 min at 38 degrees C can be appreciated.

Published

1990

2. Flow cytometric analysis of the effects of 0.4 MeV fission neutrons on mouse spermatogenesis.

Author

Spanò M, Pacchierotti F, Mauro F, Quaggia S, and Uccelli R

Subjects

Animals, Cell Survival radiation effects, DNA analysis, Dose-Response Relationship, Radiation, Flow Cytometry, Male, Mice, Neutrons, Organ Size radiation effects, Polyploidy, Spermatids radiation effects, Spermatocytes radiation effects, Spermatogonia radiation effects, Testis anatomy & histology, Spermatogenesis radiation effects

Abstract

(C57Bl/Cne X C3H/Cne)F1 male mice were irradiated with single acute doses of 0.4 MeV neutrons ranging from 0.05 to 2 Gy, and testis cell suspensions were prepared for cytometric analysis of the DNA content 2-70 days after irradiation. Various cell subpopulations could be identified in the control histogram including mature and immature spermatids, diploid spermatogonia and spermatocytes, tetraploid cells and cells in the S-phase. Variations in the relative proportions of different cell types were detected at each dose and time, reflecting lethal damage induced on specific spermatogenetic stages. The reduction of the number of elongated spermatids 28 days after irradiation was shown to be a particularly sensitive parameter for the cytometrical assessment of the radiosensitivity of differentiating gonia. A D0 value of 0.13 Gy was calculated and compared with data obtained after X-irradiation, using the same experimental protocol. In the latter case a biphasic curve was obtained over the dose range from 0.25 to 10 Gy, possibly reflecting the existence of some cell population heterogeneity. RBE values were estimated at different neutron doses relative to the radiosensitive component of the X-ray curve, and ranged from 3.3 to 4, in agreement with data in the literature. Genotoxic effects were monitored 7 days after irradiation by a dose-dependent increase of the coefficient of variation (CV) values of the round spermatid peak, reflecting the induction of numerical and structural chromosome aberrations, and 14 or 21 days after irradiation by the detection of diploid elongated spermatids, probably arising from a radiation-induced complete failure of the first or second meiotic division.

Published

1987

3. Cytotoxic effects of benzene on mouse germ cells determined by flow cytometry.

Author

Spanò M, Pacchierotti F, Uccelli R, Amendola R, and Bartoleschi C

Subjects

Animals, Body Weight drug effects, DNA analysis, DNA metabolism, Dose-Response Relationship, Drug, Flow Cytometry, Germ Cells metabolism, Male, Mice, Mice, Inbred C3H, Mice, Inbred C57BL, Organ Size drug effects, Testis metabolism, Time Factors, Benzene toxicity, Germ Cells drug effects, Spermatogenesis drug effects, Testis drug effects

Abstract

Flow cytometric (FCM) DNA content measurements were performed on testicular monocellular suspensions obtained from mice exposed per os to 0, 1, 2, 4, 6, and 7 ml/kg body weight of benzene in order to investigate its cytotoxic action on germ cells. The effects of benzene were measured 7, 14, 21, 28, and 70 d after treatment. Benzene had no effect on testis weight, but FCM analysis showed the relative percentages of some cell subpopulations (tetraploid and haploid cells) to be different from the control pattern, indicating the occurrence of some cytotoxic damage to differentiating spermatogonia. These data demonstrate that spermatogenesis is sensitive to benzene single exposures as evidenced by an altered cell ratio of testicular cell types.

Published

1989

4. Effects of L-acetylcarnitine (LAC) on the post-injury recovery of mouse spermatogenesis monitored by flow cytometry. 1. Recovery after X-irradiation.

Author

Amendola R, Bartoleschi C, Cordelli E, Mauro F, Uccelli R, and Spanò M

Subjects

Animals, Flow Cytometry, Male, Mice, Mice, Inbred Strains, Spermatogenesis radiation effects, Testis cytology, Testis drug effects, Time Factors, Acetylcarnitine pharmacology, Carnitine analogs & derivatives, DNA analysis, Spermatogenesis drug effects, Testis radiation effects

Abstract

L-acetylcarnitine plays a key role in sperm metabolism and in the whole spermatogenetic process. In the present work, the influence of L-acetylcarnitine, administered i.p. (100 mg/kg body weight), on the recovery processes of mouse spermatogenesis after local acute irradiation with 10 Gy X-rays has been investigated. The effects were monitored 28, 35, 40, 45, 50, 55, and 60 days after irradiation by flow cytometric analysis of cellular DNA content. In the LAC-treated animals, the fraction of tetraploid cells is higher at 28 (p less than 0.05) and 45 days (p less than 0.02). Corresponding with the timing of the stages of murine spermatogenesis, the round spermatid fraction is higher at 45 days (p less than 0.1) and the elongated spermatid fraction is higher at 50 days (p less than 0.1) after irradiation. In addition, the LAC-treated animals show a faster recovery throughout the maturation process, from tetraploid to round and elongated spermatids. These results indicate that the presence of exogenous LAC could enhance the recovery of spermatogonial cells.

Published

1989

5. Cytotoxic effects of benzene on mouse germ cells determined by flow cytometry

Author

Pacchierotti, F., Spano, M., Amendola, R., Bartoleschi, C. Bartoleschi, and Uccelli, R.

Subjects

MICE, SPERMATOGENESIS, FLOW cytometry, BENZENE, OCCUPATIONAL hazards

Published

1989