Cellular distribution of translationally controlled tumor protein in rat and human testes.

In a recent proteomic study we identified 53 spermatogonial proteins among which was the translationally controlled tumor protein (TCTP). This is a protein previously reported as being implicated in proliferation events in normal and tumoral tissues that had never previously been seen in the testis. The present study was aimed at establishing the complete cellular distribution of TCTP and its transcript and the ontogenetic expression of this gene within the testis. Using an immunohistochemistry technique, an intense TCTP signal was detected in gonocytes (the prespermatogonia) in the fetal rat testis and in spermatogonia within adult human and neonatal and adult rat testes. Meiotic spermatocytes and postmeiotic haploid spermatids were also strongly immunostained in a stage-dependent manner in human and rat testes. In addition, different levels of TCTP expression were also observed in the testicular somatic cells, with strong expression in Leydig cells and peritubular cells, and weak expression in Sertoli cells. Western and Northern blot analyses confirmed the presence of TCTP at all ages studied, with higher levels of RNA expression at 9 and 20 d postpartum, when spermatogonia and primary spermatocytes represent the highest proportion of germ cells: it was also confirmed that TCTP is present in all populations of isolated testicular cells. A transcript of 0.85 kb corresponding to TCTP, was expressed at all ages studied. This transcript was found to be expressed strongly in spermatogonia, somewhat less in isolated Leydig, resident macrophage, peritubular and Sertoli cells, weakly in the primary spermatocytes but not at all in spermatids. Interestingly, in the latter, a different transcript of 1.1 kb was present. The same 1.1 kb transcript appeared in testis extracts from 35 days postpartum onwards, corresponding to an age when spermatids accumulate within the tubules. Of note is that resident macrophages were found to express both the 0.85 and the 1.1 kb transcripts. We conclude that the strong expression of TCTP in spermatogonia makes it highly likely that the protein plays a significant role in spermatogenesis.

Radiation effect on rat Sertoli cell function in vitro and in vivo.

PURPOSE: To investigate the response of Sertoli cell function to 60Co gamma-rays. MATERIALS AND METHODS: Rat Sertoli cells were exposed in vitro and in vivo to 60Co gamma-rays in the dose range 3 Gy to 48 Gy and at 3 Gy and 6 Gy respectively. Cell viability and transferrin and IL-6 production were measured at different times following irradiation. RESULTS: This study confirms the resistance of in vitro irradiated rat Sertoli cells in the dose range 3 Gy to 48 Gy in terms of cell number. Radiation had no effect on the IL-1 activity of Sertoli cells. However, the experiments show that despite the absence of a macroscopic effect, Sertoli cells respond to ionizing radiation by increasing transferrin secretion, transferrin response to (Bu)2cAMP stimulation and IL-6 activity. CONCLUSIONS: Transferrin is involved in the transport of iron into germ cells and in cell differentiation. IL-6 is a potent inhibitor of meiotic DNA synthesis. Radio-induced transferrin and IL-6 could play a role in the protection of germ cells and could explain, in part, the resistance of Sertoli cells to radiation.

The Co-culture of Sertoli Cells and Germ Cells: Applications in Toxicology.

Spermatogenesis is a very complex process by which male germ cells differentiate into mature spermatozoa. In this regard, the local regulation of spermatogenesis can be considered as a particular cellular achievement. This sophisticated communication network has its weak points, such that the dysfunctionment of one cell type propagates to all other cell types as a cascade. This explains the particular vulnerability of the testis to environmental factors, and more specifically drugs and xenobiotics, and the general difficulty encountered by the toxicologist in identifying the testicular cell target of a given toxicant and hence its precise mode of action. More or less complex culture systems of isolated testicular cells have been developed over the past decades which represent very useful tools for the toxicologist. Among the different testicular cell types, Sertoli and Leydig cells, have been the ones most usually used for the in vitro analysis of toxic compounds. While Sertoli cells are used in vitro for mechanistic toxicology studies, the extreme fragility of germ cells prevents their culture for that purpose. However, Sertoli and germ cells can be cultured together for short periods of time. This review presents the different in vitro testicular systems at disposal and provides examples of mechanistic studies undertaken to verify and deepen in vivo observations on the targets to reproductive toxicants.

NRD convertase: a putative processing endoprotease associated with the axoneme and the manchette in late spermatids.

N-arginine dibasic convertase is a novel metalloendopeptidase which selectively cleaves at the N terminus of arginine residues in paired basic amino acids. Although present in brain and several other tissues, NRD convertase is particularly abundant in testis, where its expression appeared to be restricted to germ cells. Low levels of both mRNA and its corresponding protein were detected early in spermatogenesis. However, a marked accumulation of the protein was observed during late steps (14 to 19) of spermiogenesis. By electron microscopy, the NRD convertase immunoreactivity was localized in the cytoplasm of elongating and elongated spermatids, with a noticeable concentration at the level of two microtubular structures, i.e. the manchette and the axoneme. These observations strongly support the hypothesis that NRD convertase is involved in processing events potentially associated with the morphological transformations occurring during spermiogenesis.

Characterization of tonoplast-enriched vesicles isolated by gradient density fractionation of suspension-cultured cells.

A tonoplast-enriched microsomal fraction was isolated from Catharanthus roseus cells. It was characterized by structural and functional criteria. This fraction presented a homogeneous size distribution as shown by quasi-elastic light scattering and a homogeneous density on self-generated gradients of Percoll. The mean diameter of the vesicles was estimated to be 0.30 micron and the buoyant density around 1.04 g/ml. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis analysis of its polypeptide pattern was in good agreement with the one obtained for tonoplast purified from isolated vacuoles. According to enzymatic assays and inhibition tests, this fraction possessed pyrophosphate and ATP-dependent proton pumps and very low contamination by submitochondrial particles, endoplasmic reticula and Golgi membranes. In light of our previous published results on tonoplast purified from isolated vacuoles, the very low extent of AMP hydrolysis by the microsomal fraction is interpreted as supplementary proof in favor of a tonoplast-enriched fraction.

Dinoflagellate luminescence: purification of a NAD(P)H-dependent reductase and of its substrate.

The soluble enzymatic luminescent system of the dinoflagellate Pyrocystis lunula (luciferase-luciferin) is coupled with an enzymatic NAD(P)H-dependent reaction. The enzyme is a soluble reductase (Mr 47,000) which catalyzes, in the presence of NAD(P)H, the reduction of a molecule called P630. Reduced P630 has the same spectral characteristics as the purified luciferin. The luciferase can oxidize this reduced molecule with a light emission at 480 nm. These observations suggest that reduced P630 is a luciferin molecule. The oxidized form seems, in these conditions, to be the precursor of luciferin.

Does a proton-pumping ATPase exist in the tonoplast?

In order to account for the accumulation of metabolites in plant vacuoles, the existence of a proton-pumping ATPase has been widely suggested in the literature. The demonstration of such a tonoplast-bound ATPase was merely based on the characterization of a nitrate-sensitive microsomal fraction. In some examples, this ATPase activity has been evidenced on vacuole preparations obtained under conditions which were criticized by Boller. The application of the reverse phase high-performance liquid chromatography method (RP-HPLC) to the simultaneous separation of adenine nucleotides, in the presence of tonoplast vesicles isolated from Catharanthus roseus, showed results not necessarily correlated with the ATPase hypothesis. Moreover, in light of the H+-quenching of quinacrine fluorescence observed during ATP hydrolysis by vacuoles or tonoplast vesicles, the existence of a proton-pumping ATPase may be questioned.

Design of a chemiluminescent and bioluminescent photometer.

An apparatus for chemi- and bioluminescence measurements is described. The main features are in high sensitivity: for example, 5 10(-12) M adenosine triphosphate, 5 10(-7) M glucose, 2 10(-9) M perhydrol and 4 10(-13) M peroxidase are easily detected; its fast mixing time and the possibility of injecting a reactant, at any time, enabling kinetic studies. Moreover, its compactness and 12 V battery supply allow measurements outside of laboratories.

Inactivation of alpha-chymotrypsin by new bifunctional reagents: halomethylated derivatives of dihydrocoumarins.

alpha-Chymotrypsin is rapidly and completely inactivated by a series of halomethylated derivatives of dihydrocoumarins at pH 7 and 25 degrees. The inactivation is pH-dependent and optimal at neutral pH; it is also more or less complete depending on the excess of inhibitor with respect to the enzyme. These compounds are substrates for alpha-chymotrypsin and, during the catalytic process, a latent alkylating function of the reagent is activated at the active site of the enzyme and reacts with some vicinal nucleophilic amino acid residues. The stoichiometry of the reaction of the corresponding radioactive reagents with the enzyme is slightly superior to one, but one histidine residue of alpha-chymotropsin is mainly modified. This histidine is identified as histidine-57 by the diagonal peptide mapping method. In comparison with other reagents, the efficiency of these suicide substrates" and particularly that one of a derivative (compound 2) carrying a substrate-like side chain is found to be very high.

Inactivation of proteases and esterases by halomethylated derivatives of dihydrocoumarins.

A series of halomethylated derivatives of dihydrocoumarins has been found to inhibit irreversibly proteases and esterases. alpha-Chymotrypsin, subtilish, elastase are rapidly inactivated in the presence of these compounds, while trypsin, kallicrein, papain are inhibited more slowly. Esterases like acetylcholinesterase and butyrylcholinesterase also lose activity in their presence. Two structural features of these inactivators are essential for inhibition: a reactive cis-ester function and an alkylating function. Analogues of these derivatives having only one of these characteristics are inefficient. Therefore it is suggested that the efficiency of these bifunctional reagents is due to their character of potential "suicide substrates".

Resonance Raman spectroscopic studies of the interactions between trypsin and a competitive inhibitor.

Raman spectroscopy was used to study the interactions between bovine trypsin and a competitive inhibitor. For this purpose, a chromophoric substrate analogue, 4-amidino-4'-dimethylamine azobenzene, was synthesized. This compound competitively inhibits the enzyme with a 1:1 stoichiometry and an inhibition constant Ki of 2.3 muM at pH 6.08 and 15 degrees. Resonance Raman spectra in aqueous solution of free or enzyme-bound inhibitor were analyzed. The main spectral changes observed upon enzyme-inhibitor complex formation were changes in the relative intensities of four bands (1171, 1206, 1315, 1608 cm-1) while no large frequency shifts occurred. The binding of the inhibitor molecule to the enzyme did not induce a twisting of the phenyl groups around the N=N bond. Some modifications of the band widths are interpreted in terms of a restriction of rotational motions in the inhibitor molecule. The possible involvement of specific interactions between trypsin and the benzamidinium ion part of the inhibitor molecule is discussed.