Abstract
We have investigated the possibility that transgenerational effects from preconceptional paternal irradiation (PPI) may render offspring more vulnerable to secondary exposure to an unrelated carcinogen. 239Pu (0, 128 or 256 Bq g(-1)) was administered by intravenous injection to male mice, 12 weeks before mating with normal females. Two strains of mouse were used -- CBA/H and BDF1. Haemopoietic spleen colony-forming units (CFU-S) and fibroblastoid colony-forming units (CFU-F), a component of their regulatory microenvironment, were assayed independently in individual offspring at 6, 12 and 19 weeks of age. Bone marrow and spleen from each of these mice were grown in suspension culture for 2 or 7 days for assessment of chromosomal aberrations. Female BDF1 were injected with methyl-nitroso-urea (MNU) as a secondary carcinogen at 10 weeks of age and monitored for onset of leukaemia/lymphoma. Mean values of CFU-S and CFU-F were unaffected by preconceptional paternal plutonium-239 (PP-239Pu), although for CFU-F in particular there was an apparent increase in variation between individual animals. There was significant evidence of an increase in chromosomal aberrations with dose in bone marrow but not in spleen. By 250 days, 68% of MNU-treated control animals (no PPI) had developed thymic lymphoma (62%) or leukaemia (38%). The first case arose 89 days after MNU administration. In the groups with PPI, leukaemia/lymphoma developed from 28 days earlier, rising to 90% by 250 days. Leukaemia (65%) now predominated over lymphoma (35%). This second generation excess of leukaemia appears to be the result of PPI and may be related to inherited changes that affect the development of haemopoietic stem cells.
Highlights
Leukaemia (65%) predominated over lymphoma (35%). This second generation excess of leukaemia appears to be the result of preconceptional patemal irradiation (PPI) and may be related to inherited changes that affect the development of haemopoietic stem cells
At the higher dose of "9Pu. the mice W ere slow er to mate and for the BDF1 a second batch of pairings had to be introduced in order to obtain sufficient litters. there Aere no strnificant differences in the size of those litters born
Our results suggest that such destabilization can be transmitted through the germ line and expressed as elevated levels of chromosome aberrations in bone marrow cells of PPI offspring
Summary
Experiments 'Aere conducted in tx-o strains of mouse: (i) DBA2 male mice. mated x-ith C57B16 females to generate a BDF1 hxbrid. and (ii) inbred CBA/H mice of both sexes. (ii) inbred CBA/H mice of both sexes. Experiments 'Aere conducted in tx-o strains of mouse: (i) DBA2 male mice. Mated x-ith C57B16 females to generate a BDF1 hxbrid. They A-ere treated and maintained under Home Office Licence according to the provisions of the U'nited Kingdom. Procedures for preparation of the injection solutions 'were as previously described (Schofield et al 1986). W-as injected intraxenously in approximatelx 0.2-ml units containing 128 or 256 Bq g-- body wxeioht. Each mouse >-as w-eighed indixidually and injected . Comparable citrate carrier solutions 'ere made up for control group injections
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