Induction of precocious sex reversal in aquaculture: effects of methyltestosterone treatment on gonadal sex of yearling longtooth grouper (Epinephelus bruneus)

Groupers, highly valued fish globally, exhibit sex change from female to male during adulthood, posing challenges in obtaining wild males for aquaculture. Inducing female-to-male sex reversal in juvenile groupers can streamline breeding efforts. This study used 17a-Methyltestosterone (MT)-loaded cholesterol pellets to treat one-year-old longtooth groupers (Epinephelus bruneus) and induce small functional males. Gonadal sexuality and male functionality were assessed after one to two months. Initial gonadal changes included efferent duct differentiation. High-dose MT-treated fish exhibited active spermatogenesis. However, no spermiation was observed. This highlights MT's potential for sex reversal but not for complete testicular function. These findings have implications for grouper aquaculture and the management of sex change. Further research should explore methods to optimize functional male induction for sustainable breeding practices

Ordered association of helicase loader proteins with the Bacillus subtilis origin of replication in vivo

January 1, 2011The essential proteins DnaB, DnaD and DnaI of Bacillus subtilis are required for initiation, but not elongation, of DNA replication, and for replication restart at stalled forks. The interactions and functions of these proteins have largely been determined in vitro based on their roles in replication restart. During replication initiation in vivo, it is not known if these proteins, and the replication initiator DnaA, associate with oriC independently of each other by virtue of their DNA binding activities, as a (sub)complex like other loader proteins, or in a particular dependent order. We used temperature-sensitive mutants or a conditional degradation system to inactivate each protein and test for association of the other proteins with oriC in vivo. We found that there was a clear order of stable association with oriC; DnaA, DnaD, DnaB, and finally DnaI-mediated loading of helicase. The loading of helicase via stable intermediates resembles that of eukaryotes and the established hierarchy provides several potential regulatory points. The general approach described here can be used to analyse assembly of other complexes.Netherlands Organization for Scientific Research (Rubicon fellowship)National Institutes of Health (U.S.) (Public Health Service Grant GM41934

Characteristics of Urban Culture from a Viewpoint of the Railway Station Hotel

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DESIGN THEME IN ENTERTAIMENT AND ACCOMMODATION FACILITIES

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Two forms of ribosomal protein L2 of Escherichia coli that inhibit DnaA in DNA replication

We purified an inhibitor of oriC plasmid replication and determined that it is a truncated form of ribosomal protein L2 evidently lacking 59 amino acid residues from the C-terminal region encoded by rplB. We show that this truncated form of L2 or mature L2 physically interacts with the N-terminal region of DnaA to inhibit initiation from oriC by apparently interfering with DnaA oligomer formation, and the subsequent assembly of the prepriming complex on an oriC plasmid. Both forms of L2 also inhibit the unwinding of oriC by DnaA. These in vitro results raise the possibility that one or both forms of L2 modulate DnaA function in vivo to regulate the frequency of initiation

Highly organized DnaA–oriC complexes recruit the single-stranded DNA for replication initiation

In Escherichia coli, the replication origin oriC consists of two functional regions: the duplex unwinding element (DUE) and its flanking DnaA-assembly region (DAR). ATP-DnaA molecules multimerize on DAR, unwinding DUE for DnaB helicase loading. However, DUE-unwinding mechanisms and functional structures in DnaA–oriC complexes supporting those remain unclear. Here, using various in vitro reconstituted systems, we identify functionally distinct DnaA sub-complexes formed on DAR and reveal novel mechanisms in DUE unwinding. The DUE-flanking left-half DAR carrying high-affinity DnaA box R1 and the ATP-DnaA-preferential DnaA box R5, τ1-2 and I1-2 sites formed a DnaA sub-complex competent in DUE unwinding and ssDUE binding, thereby supporting basal DnaB loading activity. This sub-complex is further subdivided into two; the DUE-distal DnaA sub-complex formed on the ATP–DnaA-preferential sites binds ssDUE. Notably, the DUE-flanking, DnaA box R1–DnaA sub-complex recruits DUE to the DUE-distal DnaA sub-complex in concert with a DNA-bending nucleoid protein IHF, thereby promoting DUE unwinding and binding of ssDUE. The right-half DAR–DnaA sub-complex stimulated DnaB loading, consistent with in vivo analyses. Similar features are seen in DUE unwinding of the hyperthermophile, Thermotoga maritima, indicating evolutional conservation of those mechanisms