Overcoming Radical Stability Order via DABCO-Triggered Desulfurization: Visible-Light-Promoted 1,2,4-Trifunctionalization of Butenyl Benzothiazole Sulfone with Thiosulfonate.

A radical 1,2,4-trifunctional reaction of thiosulfonate to unactivated olefin is achieved by a migration strategy under mild conditions. In this reaction, the more unstable primary free radicals are in situ generated after the migration of heteroaryl groups in the presence of DABCO. This trifunctionalization of unactivated olefins involves two C-S bond formations and one C-C bond formation.

Effective Separation of Human Milk Glycosides using Carbon Dioxide Supercritical Fluid Chromatography.

Carbohydrate purification remains problematic due to the intrinsic diversity of structural isomers present in nature. Although liquid chromatography-based techniques are suitable for analyzing or preparing most glycan structures acquired either from natural sources or through chemical or enzymatic synthesis, the separation of regioisomers or linkage isomers with a clear resolution remains challenging. Herein, a carbon dioxide supercritical fluid chromatography (SFC) method was devised to resolve 18 human milk glycosides: oligomers (disaccharides to hexasaccharides), fucosylated regioisomers (lacto-N-fucopentaose I, III, and V; lacto-N-neofucopentaose V; lacto-N-difucohexaose III; blood group H1 antigen; and TF-LNnT), and connectivity isomers (lacto-N-tetraose/lacto-N-neotetraose and para-lacto-N-hexaose/para-lacto-N-neohexaose/type-1 hexasaccharide). The analysis of these glycosides represents a major limitation associated with conventional carbohydrate analysis. The unprecedented resolution achieved by the SFC method indicates the suitability of this key technology for revealing complex human milk glycomes.

Comparative transcriptome analysis reveals an early gene expression profile that contributes to cold resistance in Hevea brasiliensis (the Para rubber tree).

The rubber tree (Hevea brasiliensis Muell. Arg) is a tropical, perennial, woody plant that is susceptible to cold stress. In China, cold stress has been found to severely damage rubber plants in plantations in past decades. Although several Hevea clones that are resistant to cold have been developed, their cold hardiness mechanism has yet to be elucidated. For the study reported herein, we subjected the cold-resistant clone CATAS93-114 and the cold-sensitive clone Reken501 to chilling stress, and characterized their transcriptomes at 0, 2, 8 and 24 h after the start of chilling. We found that 7870 genes were differentially expressed in the transcriptomes of the two clones. In CATAS93-114, a greater number of genes were found to be up- or downregulated between 2 h and 8 h than in Reken501, which indicated a more rapid and intensive response by CATAS93-114 than by Reken501. The differentially expressed genes were grouped into seven major clusters, according to their Gene Ontology terms. The expression profiles for genes involved in abscisic acid metabolism and signaling, in an abscisic acid-independent pathway, and in early signal perception were found to have distinct expression patterns for the transcriptomes of the two clones. The differential expression of 22 genes that appeared to have central roles in response to chilling was confirmed by quantitative real-time PCR.

Functional Characterization of Hevea brasiliensis CRT/DRE Binding Factor 1 Gene Revealed Regulation Potential in the CBF Pathway of Tropical Perennial Tree.

Rubber trees (Hevea brasiliensis) are susceptible to low temperature and therefore are only planted in the tropical regions. In the past few decades, although rubber trees have been successfully planted in the northern margin of tropical area in China, they suffered from cold injury during the winter. To understand the physiological response under cold stress, we isolated a C-repeat binding factor 1 (CBF1) gene from the rubber tree. This gene (HbCBF1) was found to respond to cold stress but not drought or ABA stress. The corresponding HbCBF1 protein showed CRT/DRE binding activity in gel shift experiment. To further characterize its molecular function, the HbCBF1 gene was overexpressed in Arabidopsis. The HbCBF1 over expression (OE) line showed enhanced cold resistance and relatively slow dehydration, and the expression of Arabidopsis CBF pathway downstream target genes, e.g. AtCOR15a and AtRD29a, were significantly activated under non-acclimation condition. These data suggest HbCBF1 gene is a functional member of the CBF gene family, and may play important regulation function in rubber tree.

TiO2 nanotube array-graphene-CdS quantum dots composite film in Z-scheme with enhanced photoactivity and photostability.

The most efficient solar energy utilization is achieved in natural photosynthesis through elaborate cell membrane with many types of molecules ingeniously transferring photogenerated electrons to reactants in a manner similar to the so-called Z-scheme mechanism. However, artificial photosynthetic systems based on semiconductor nanoparticles are inevitably accompanied by undesired non-Z-scheme electron transfer and back reactions, which adversely affect the photoactivity and photostability of the systems. Herein, we report on a novel Z-scheme system with an electrochemically converted graphene (GR) film as the electron mediator interlayer contacted with both TiO2 nanotube (TNT) array and CdS quantum dots (CdS QDs) on two sides. The obtained TiO2 nanotube array-graphene-CdS quantum dots (TNT-GR-CdS) composite film shows higher photoelectric response and photocatalytic activities than other bare TNT, TNT-CdS, TNT-GR, and TNT-CdS-GR. Moreover, compared to TNT-CdS, the activity stability is significantly improved, and the residual amount of Cd element in reaction solution is reduced ∼8 times over TNT-GR-CdS. Various measurements of photoelectrochemistry and radicals reveal that the enhanced photoactivity and photostabilities of TNT-GR-CdS are due to the efficient spatial separation of the photogenerated electron-hole pairs and the restricted photocorrosion of CdS via an efficient Z-scheme mechanism under simulated sunlight.

Photoelectrocatalytic degradation of rhodamine B on TiO2 photonic crystals.

As the inverse-opal structure facilitates the separation of electron-hole pairs and electron transfer, it may generate many radical species with strong oxidation capability. When a low bias voltage was applied on the TiO2 electrodes with inverse-opal structure, they exhibited more excellent photoelectrochemical properties and photoelectrocatalytic activity than TiO2 film under simulated solar light irradiation. When different types of active species scavengers were added, the different performances of TiO2 photonic crystals in rhodamine B degradation showed that besides ˙OH and holes, which were the main active species in the photocatalysis, O2˙(-) played a vital role in the photoelectrocatalytic degradation process. Furthermore, the stronger signal of ˙OH-trapping photoluminescence and the variation in the concentration of nitroblue tetrazolium reflected that more ˙OH and O2˙(-) could be generated in the photoelectrocatalysis than that in the photocatalysis, and O2˙(-) was partially obtained from the cathode surface. At last, the roles active species played in the photoelectrocatalytic and photocatalytic processes were compared, and the possible degradation mechanisms of TiO2 photonic crystals in photoelectrocatalytic and photocatalytic systems were put forward, which could provide a good insight into the mechanism of photoelectrocatalytic degradation on TiO2 photonic crystals.

[Marrow mesenchymal stem cell transplantation with sodium alginate gel for repair of spinal cord injury in mice].

OBJECTIVE: To investigate the effects of sodium alginate gels on marrow mesenchymal stem cell transplantation for repair of spinal cord injury (SCI) in mice. METHODS: In the present study, effects of different sterilization methods and concentrations of sodium alginate gels were examined. Marrow mesenchymal stem cells (mMSCs) were isolated from mice and cultured. Cells were cultured with sodium alginate gels and MTT assay was applied to determine the cell viability. Mice spinal cord injury was induced by spinal cord transection. mMSCs were transplanted into the cavity of injured spinal cord with sodium alginate gels. The effects of sodium alginate gel were assessed by BMS scales and immunofluorescence staining for NF-200. RESULTS: Compared with liquid form, solid form sodium alginate gel prepared with high pressure vapor sterilization had a better effect on cell viability. SCI mice treated with 10 % sodium alginate gel and mMSCs achieved higher score in BMS scale as well as higher expression of NF-200 compared with the untreated SCI group. CONCLUSION: Sodium alginate gel prepared with solid form sterilization induces mMSCs proliferation and thus can be used as the carrier of stem cell in treatment of SCI.