Mutagenic effects of selected trichothecene mycotoxins and their combinations with aflatoxin B1

The authors focused on the amplification of data on the mutagenicity of selected trichothecene mycotoxins (T-2 toxin, vomitoxin) and their combination with aflatoxin B₁,which is known to be a strong mutagen. Mutagenic activity was investigated using the Ames test in a prokaryote model at low doses (close to 0.1 LD₅₀). Whereas the individual trichothecene mycotoxins (T-2 toxin, vomitoxin) did not show any mutagenic activity in the test systems mentioned, in combination with AFB₁, or as a combination of all three mycotoxins, they showed a mutagenic effect significantly greater than AFB₁ alone in the Ames test (in strain TA98 at all concentrations) as well as in the micronucleus test (combination of T-2 toxin with AFB₁).

Protective role of methanol extracts of Gentiana asclepiadea L. and G. cruciata L. against genotoxic damage induced by ethyl methanesulfonate

The methanol extracts from the underground and aerial part of the two species of Gentiana genus, Gentiana asclepiadea L. and Gentiana cruciata L. from Serbia, were investigated for their antigenotoxic activity against wellestablished mutagenic agent ethyl methanesulfonate (EMS) using the in vivo sexlinked recessive lethal (SLRL) test on Drosophila melanogaster. For this purpose, three days old Canton S males were treated with the potent mutagen EMS in concentration of 0.75 ppm, alone and combined with methanol extracts obtained from underground or aerial part of G. asclepiadea and G. cruciata in concentration of 5%, separately. Although EMS in concentration of 0.75 ppm increased the mutation frequency in all three broods, post-treatments with methanol extracts obtained from the underground and aerial part of G. asclepiadea and G. cruciata in concentration of 5%, respectively, drastically reduced the frequency of sex-linked recessive lethal mutations induced by EMS. Compared to the sucrose, as a negative control, methanol extract obtained from underground part of G. cruciata showed the most potent antigenotoxic activity. Extracts from the underground and aerial part of the two species of Gentiana genus, G. asclepiadea L. and G. cruciata L. from Serbia used in our experiments showed a clear antimutagenic effect, reducing the frequency of mutations induced by a strong mutagen such as EMS.

Molecular mechanisms of cadmium induced mutagenicity

Cadmium is a human carcinogen of worldwide concern because it accumulates in the environment due to its extremely long half-life. Its compounds are classified as human carcinogens by several regulatory agencies. Cadmium affects cell proliferation, differentiation, apoptosis and other cellular activities and can cause numerous molecular lesions that would be relevant to carcinogenesis. For a long time cadmium has been considered as a non-genotoxic carcinogen, as it is only weakly mutagenic in bacterial and mammalian cell test systems. Recently, we presented evidence that when assayed in a test system, in which both intragenic and multilocus mutations can be detected, cadmium acts as a strong mutagen which induces predominantly multilocus deletions. In this review, we discuss two mechanisms that play an important role in cadmium mutagenicity: (i) induction of reactive oxygen species (ROS); and (ii) inhibition of DNA repair. Experimental evidence suggests that cadmium at low, for environmental exposure relevant concentrations, induces mutations by inducing oxidative DNA damage and that it decreases genetic stability by inhibiting the repair of endogenous and exogenous DNA lesions, which in turn increase the probability of mutations and consequently cancer initiation by this metal.

Introduction and Removal of Disinfection Byproducts and Mutagenic Activity by Chemical and Photolytic Treatments

Samples from four different raw water sources were treated with various disinfectants and subjected to chemical analyses and mutagenicity assays. The following disinfectants were used: chlorine (Cl2), chlorine dioxide (ClO2), monochloramine (NH2Cl), ozone (O3), ultraviolet radiation (UV), and combinations of Cl2/ClO2, O3/Cl2, UV/Cl2, and UV/O3/Cl2. The samples were analysed for adsorbable organic halogens (AOX), chloroform (CHCl3), carboxylic acids, volatile organics, chlorite, the strong mutagen 3-chloro-4 (dichloromethyl)-5-hydroxy-2 (5H)-furanone (MX), and mutagenic activity (as detected by the Ames test). Humic lake water which had been treated with the combination UV/Cl2 exhibited a higher level of mutagenicity and higher concentrations of MX and CHCl3 than water treated with Cl2 alone. The same observation was made for the mutagenicity and the CHCl3 concentration in waters preoxidized with low doses of O3 and UV/O3, respectively. When higher doses of these powerful oxidants were used in the pretreatment step, the level of mutagenicity, MX and CHCI3 were lower than in water chlorinated without pretreatment. The combination UV/O3 was found to be more efficient than O3 alone in destroying the precursor material to the mutagenic compounds and chloroform. The higher the proportion of ClO2 in the combined Cl2/ClO2 process, the lower the levels of mutagenicity, MX, CHCl3, and AOX. The production of inorganic chlorite increased with a higher proportion of ClO2. Aldehydes, n-alkanes, and low molecular-weight carboxylic acids were identified as byproducts following UV treatment of humic lake water. The mutagenic activity (per amount of DOC) was approximately similar after chlorination of humic rich surface- and ground waters as after chlorination of waters from the rivers Meuse and Rhine, containing relatively low amounts of humic matter. The precursors to MX were found to be more abundant in the humic waters than in the river waters.