Asparagine and regulation of photoinduced rhythm in Penicillium claviforme

A photosensitive reaction involved in the expression and regulation of the endogenous sporulation rhythm in Penicillium claviforme Bainier CBS 126-23 has been described earlier by our team. The present work shows that asparagine plays a central role in this periodic system. The 24–26 h periodicity, which becomes desynchronized over a few days, was affected by supplying asparagine (1 to 25 m M ). a) The rhythm remained synchronized for at least 3 weeks, for all the asparagine concentrations used, b) The period increased successively from one cycle to the next (from 35±3 h to 73±8 h over 6 cycles) for 1 m M asparagine. This period lengthening became less and less accentuated as the asparagine concentration was increased. At ≥10 m M , the period was stable; it was 33±5 h for 10 m M and 22±1.5 h for 25 m M asparagine. Otherwise asparagine could not elicit rhythmicity in darkness or in dim continuous light (≤5 μW m⁻²).     

Brca1 in immunoglobulin gene conversion and somatic hypermutation

Defects in Brca1 confer susceptibility to breast cancer and genomic instability indicative of aberrant repair of DNA breaks. Brca1 was previously implicated in the homologous recombination pathway via effects on the assembly of recombinase Rad51. Activation-induced cytidine deaminase (AID) deaminates C to U in B lymphocyte immunoglobulin (Ig) DNA to initiate programmed DNA breaks. Subsequent uracil-glycosylase mediated U removal, and perhaps further processing, leads to four known classes of mutation: Ig class switch recombination that results in a region-specific genomic deletion, Ig somatic hypermutation that introduces point mutations in Ig V-regions, Ig gene conversion in vertebrates that possess Ig pseudo-V genes, and translocations common to B cell lymphomas. We tested the involvement of Brca1 in AID-dependent Ig diversification in chicken DT40 cells. The DT40 cell line diversifies IgVlambda mainly by gene conversion, and less so by point mutation. Brca1-deficiency caused a shift in Vlambda diversification, significantly reducing the proportion of gene conversions relative to point mutations. Thus, Brca1 regulates AID-dependent DNA lesion repair. Interestingly, while Brca1 is required to recruit ubiquitinated FancD2 to DNA damage, the phenotype of Brca1-deficient DT40 differs from the one of FancD2-deficient DT40, in which both gene conversion and non-templated mutations are impaired.     

Cyclic AMP level in relation to different conditions of sporulation rhythm regulation in Leptosphaeria michotii (West) Sacc

When Leptophaeria michotii was grown in conditions that permitted a stable periodicity of sporulation (asparagine 6.6 mM in darkness or asparagine 2.6 mM in continuous white light), the level of intracellular cyclic AMP was lower and the activity of the cyclic AMP phosphodiesterase higher in contrast to the cultures with an instable periodicity.With asparagine 6.6 mM and in darkness, theophylline (1 mM) increased the intracellular cyclic AMP level whereas caffeine (1 mM) had no effect. Theophylline (0.01 and 0.1 mM) or caffeine (0.01–1 mM) provoked a rhythm instability under these conditions. Isoproterenol (1 mM) increased the cyclic AMP level. Nevertheless, the instable rhythm observed in control fed with asparagine 2.6 mM in darkness, was partially stabilized with isoproterenol 0.01 M or 0.01–1 mM. Exogenous cyclic AMP (0.01–1 mM) provoked a complete regulation of the rhythm with asparagine 2.6 mM and a shortening of the stable period (from 27 to 21 h) when the fungus was grown on asparagine 6.6 mM.These results underlined the fact that Leptosphaeria rhythm regulation was not dependent on the cyclic AMP level only.     

Cyclic changes in translation of the mitochondrial isoenzyme account for the rhythm of aspartate aminotransferase activity in Leptosphaeria michotii

Aspartate aminotransferase in Leptosphaeria michotii has previously been shown to have an activity rhythm in constant conditions. The enzyme is present as two isofonns whose levels were quantified along the activity rhythm by ELISA, using specific polyclonal antibodies raised against polypeptides purified to a state of apparent homogeneity. The time-course of the level of the cytosolic isoform remained unchanged along the experiment. On the contrary, the cyclic variations in amount and transaminase activity (using cysteine sulfinate as substrate) of the mitochondrial isofonn gave rise to the aspartate aminotransferase activity rhythm of the fungus. The mRNA levels of the two isofonns, as determined by in vitro heterologous translation, remained monotonous along the daily cycle. These results and the sensitivity of the rhythm towards protein synthesis inhibitors are consistent with the hypothesis that the aspartate aminotransferase activity rhythm in this species is caused by some mechanism controlling the efficiency of translation of mitochondrial isoform mRNA.     

Occurrence of the mucinous differentiation antigen CA125 in genital tract and conductive airway epithelia of diverse mammalian species (rabbit, dog, monkey)

CA125 is a human tumor-associated antigen of coelomic epithelial origin. In the present study, immunohistochemical analysis of normal rabbit, dog, and monkey tissues using monoclonal antibody OC125, revealed that in these animals positive staining for CA125 is found in all tissues that produce this mucin-like glycoprotein in man, i.e., the peritoneal and pleural mesothelium, the different Müllerian-duct-derived epithelia of the female genital tract, and the epithelium of trachea, bronchi, bronchioli, and mucoserous respiratory glands; CA125 was also detected in some ductal and acinar cells of the dog mammary gland. Without trypsin treatment of sections, staining was predominantly localized on the apical cell surface of all mentioned cell types. After treatment, mucin droplets inside respiratory mucous cells were also positively stained. In all cases, staining was associated with material positive for periodic acid-Schiff (PAS) and Alcian blue. In rats, its presence could not be demonstrated. Our results show that the CA125 epitope is not restricted to man and that its expression throughout different animal species is associated with well-defined tissue compartments. The expression of the mucous differentiation antigen CA125 in several common laboratory animals provides new opportunities for the experimental study of its biological significance.