Mesoporous Technische Universiteit Delft(TUD-1)-supported chromium oxide-doped titania(Cr-TiO2) was developed as a promising photocatalyst for phenol photodegradation under visible light irradiation.Low-angle X-ra...Mesoporous Technische Universiteit Delft(TUD-1)-supported chromium oxide-doped titania(Cr-TiO2) was developed as a promising photocatalyst for phenol photodegradation under visible light irradiation.Low-angle X-ray diffraction and Fourier transform infrared spectroscopy results confirmed the amorphous and mesoporous silicate framework of TUD-1 in TUD-1-supported Cr-TiO2.The mesostructure of TUD-1 was further verified via N2 adsorption-desorption analysis,which showed a type-IV isotherm with a narrow average pore size distribution of 3.9 nm and high surface area of 490 m^2/g.Transmission electron microscopy analysis results indicated that TUD-1-supported Cr-TiO2 contained nanoparticles and porous channels.An increase in band gap energy was observed after loading Cr-TiO2 into TUD-1.Compared with that of unsupported Cr-TiO2,TUD-1-supported Cr-TiO2 showed higher photocatalytic activity for phenol degradation under visible light irradiation.The TUD-1 supported Cr-TiO2 photocatalyst with a Si/Ti molar ratio of 30 exhibited the highest photodegradation of phenol(82%) of the prepared samples.The photodegradation of phenol by the supported catalyst followed the Langmuir adsorption isotherm with first-order kinetics.展开更多
In this article,we have identified an error in the original publication of Figures 4B and 4C.The HSP82 reference lanes are misaligned with the corresponding target protein lanes.This occurred because we inadvertently ...In this article,we have identified an error in the original publication of Figures 4B and 4C.The HSP82 reference lanes are misaligned with the corresponding target protein lanes.This occurred because we inadvertently included the first lane of the immunoblot,which con-tains callus samples collected one day before BL treatment.These samples were initially used to validate callus protein expression and subsequently included as a positive control on the blot.The original uncropped blotting pictures that we used for preparing Figures 4B and 4C are provided as Figure S1 to this Correction notice.We sincerely regret this error.This correction does not affect the conclusions of the article.展开更多
Brassinosteroids(BRs)are a class of steroid hormones with great potential for use in crop improvement.De-repression is usually one of the key events in hormone signaling.However,how the stability of GSK2,the central n...Brassinosteroids(BRs)are a class of steroid hormones with great potential for use in crop improvement.De-repression is usually one of the key events in hormone signaling.However,how the stability of GSK2,the central negative regulator of BR signaling in rice(Oryza sativa),is regulated by BRs remains elusive.Here,we identify the U-box ubiquitin ligase TUD1 as a GSK2-interacting protein by yeast two-hybrid screening.We show that TUD1 is able to directly interact with GSK2 and ubiquitinate the protein.Phenotypes of the tud1 mutant are highly similar to those of plants with constitutively activated GSK2.Consistent with this finding,GSK2 protein accumulates in the tud1 mutant compared with the wild type.In addition,inhibition of BR synthesis promotes GSK2 accumulation and suppresses TUD1 stability.By contrast,BRs can induce GSK2 degradation but promote TUD1 accumulation.Furthermore,the GSK2 degradation process is largely impaired in tud1 in response to BR.In conclusion,our study demonstrates the role of TUD1 in BR-induced GSK2 degradation,thereby advancing our understanding of a critical step in the BR signaling pathway of rice.展开更多
基金the Ministry of Higher Education,Malaysia and Universiti Teknologi Malaysia(UTM) for the financial supports through Research University Grants (Q.J130000.2426.03G35 and Q.J130000.2526.10H54)
文摘Mesoporous Technische Universiteit Delft(TUD-1)-supported chromium oxide-doped titania(Cr-TiO2) was developed as a promising photocatalyst for phenol photodegradation under visible light irradiation.Low-angle X-ray diffraction and Fourier transform infrared spectroscopy results confirmed the amorphous and mesoporous silicate framework of TUD-1 in TUD-1-supported Cr-TiO2.The mesostructure of TUD-1 was further verified via N2 adsorption-desorption analysis,which showed a type-IV isotherm with a narrow average pore size distribution of 3.9 nm and high surface area of 490 m^2/g.Transmission electron microscopy analysis results indicated that TUD-1-supported Cr-TiO2 contained nanoparticles and porous channels.An increase in band gap energy was observed after loading Cr-TiO2 into TUD-1.Compared with that of unsupported Cr-TiO2,TUD-1-supported Cr-TiO2 showed higher photocatalytic activity for phenol degradation under visible light irradiation.The TUD-1 supported Cr-TiO2 photocatalyst with a Si/Ti molar ratio of 30 exhibited the highest photodegradation of phenol(82%) of the prepared samples.The photodegradation of phenol by the supported catalyst followed the Langmuir adsorption isotherm with first-order kinetics.
文摘In this article,we have identified an error in the original publication of Figures 4B and 4C.The HSP82 reference lanes are misaligned with the corresponding target protein lanes.This occurred because we inadvertently included the first lane of the immunoblot,which con-tains callus samples collected one day before BL treatment.These samples were initially used to validate callus protein expression and subsequently included as a positive control on the blot.The original uncropped blotting pictures that we used for preparing Figures 4B and 4C are provided as Figure S1 to this Correction notice.We sincerely regret this error.This correction does not affect the conclusions of the article.
基金supported by the Hainan Yazhou Bay Seed Laboratory(B21HJ0215)the National Natural Science Foundation of China(nos.U21A20208,31900177,31901534,31871587)+1 种基金the Central Publicinterest Scientific Institution Basal Research Fund(no.S2022ZD02)D.L.was funded by the China Postdoctoral Science Foundation(2020M670548).
文摘Brassinosteroids(BRs)are a class of steroid hormones with great potential for use in crop improvement.De-repression is usually one of the key events in hormone signaling.However,how the stability of GSK2,the central negative regulator of BR signaling in rice(Oryza sativa),is regulated by BRs remains elusive.Here,we identify the U-box ubiquitin ligase TUD1 as a GSK2-interacting protein by yeast two-hybrid screening.We show that TUD1 is able to directly interact with GSK2 and ubiquitinate the protein.Phenotypes of the tud1 mutant are highly similar to those of plants with constitutively activated GSK2.Consistent with this finding,GSK2 protein accumulates in the tud1 mutant compared with the wild type.In addition,inhibition of BR synthesis promotes GSK2 accumulation and suppresses TUD1 stability.By contrast,BRs can induce GSK2 degradation but promote TUD1 accumulation.Furthermore,the GSK2 degradation process is largely impaired in tud1 in response to BR.In conclusion,our study demonstrates the role of TUD1 in BR-induced GSK2 degradation,thereby advancing our understanding of a critical step in the BR signaling pathway of rice.
