Your search keyword '"Wu, Donghai"' showing total 11 results

1. Large-scale production, purification and bioactivity assay of recombinant human interleukin-6 in the methylotrophic yeast Pichia pastoris.

Author

Li H, Wang Y, Xu A, Li S, Jin S, and Wu D

Subjects

Cell Proliferation, Chemical Fractionation methods, Chromatography, DEAE-Cellulose methods, Chromatography, Gel methods, Dextrans, Humans, Interleukin-6 biosynthesis, Interleukin-6 chemistry, Lymphocytes immunology, Mass Spectrometry, Molecular Weight, Polyethylene Glycols metabolism, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins immunology, Recombinant Proteins isolation & purification, Tetrazolium Salts metabolism, Thiazoles metabolism, Gene Expression, Interleukin-6 immunology, Interleukin-6 isolation & purification, Pichia genetics, Pichia metabolism

Abstract

A DNA fragment containing the mature human interleukin (IL)-6 sequence was cloned into pPICZαA, generating a fusion protein with the alpha factor from baker's yeast and integrated into the genome of Pichia pastoris strain X-33. Recombinant yeast transformants with high-level rhIL-6 production were identified, secreting as much as 280 mg L(-1) rhIL-6 after 4 days of induction by methanol. The rhIL-6 was purified by PEG-8000 precipitation, followed by DEAE anion exchange and Sephadex G-75 gel filtration, yielding over 95% pure rhIL-6 at about 170 mg L(-1) . Mass spectrometry analysis showed that the rhIL-6 has a molecular weight of 20,908.85 Da, which is close to the mass calculated from the sequence of the protein. Functional analysis of the purified rhIL-6 using the lymphocyte proliferation assay by an MTT [3-(4,5-dimethylthiazolyl-2)-2,5-diphenyl-tetrazoliumbromide] method demonstrated a specific activity that is at least fivefold higher than the commercial rhIL-6 produced in Escherichia coli. In summary, the experimental procedure we have reported here allows us to obtain a large amount of rhIL-6 from P. pastoris suitable for subsequent biophysical studies., (© 2010 Federation of European Microbiological Societies. Published by Blackwell Publishing Ltd. All rights reserved.)

Published

2011

2. Androgen Receptor is a Negative Regulator of PRDM16 in Beige Adipocyte.

Author

Zhao, Shiting, Nie, Tao, Li, Lei, Long, Qiaoyun, Gu, Ping, Zhang, Yuwei, Sun, Wei, Lin, Zexin, Liu, Qing, Qi, Yue, Wang, Wei, Xie, Mengyuan, Loomes, Kerry, Cai, Chenleng, Wu, Donghai, and Hui, Hannah Xiaoyan

Subjects

ANDROGEN receptors, WHITE adipose tissue, BROWN adipose tissue, FAT cells, GENE expression, SEXUAL dimorphism

Abstract

PRDM16 (PR domain containing protein 16) serves as a dominant activator of brown and beige adipocyte. However, mechanisms underlying the regulation of PRDM16 expression are incompletely understood. A Prdm16 luciferase knockin reporter mouse model is generated, enabling high throughput monitoring of Prdm16 transcription. Single clonal analysis reveals high heterogeneity of Prdm16 expression in the inguinal white adipose tissue (iWAT) cells. Amongst all transcription factors, androgen receptor (Ar) shows the strongest negative correlation with Prdm16. A sex dimorphism for PRDM16 mRNA expression is present in human WAT, with female individuals exhibiting increased expression than males. Androgen‐AR signaling mobilization suppresses Prdm16 expression, accompanied by attenuated beiging in beige adipocytes, but not in brown adipose tissue. The suppressive effect of androgens on beiging is abolished upon overexpression of Prdm16. Cleavage under targets and tagmentation mapping reveals direct binding of AR within the intronic region of Prdm16 locus, whereas no direct binding is detected on Ucp1 and other browning‐related genes. Adipocyte‐selective deletion of Ar potentiates beige cell biogenesis whereas adipocyte‐specific overexpression of AR attenuates white adipose beiging. This study highlights an essential role of AR in negative regulation of PRDM16 in WAT and provides an explanation for the observed sex difference in adipose beiging. [ABSTRACT FROM AUTHOR]

Published

2023

3. Enhanced differentiation of human pluripotent stem cells into cardiomyocytes by bacteria-mediated transcription factors delivery.

Author

Jin, Yongxin, Liu, Ying, Li, Zhenpeng, Santostefano, Katherine, Shi, Jing, Zhang, Xinwen, Wu, Donghai, Cheng, Zhihui, Wu, Weihui, Terada, Naohiro, Jin, Shouguang, and Bai, Fang

Subjects

PLURIPOTENT stem cells, CELL differentiation, HEART cells, BACTERIAL genetics, GENE expression, GENETIC transcription

Abstract

Virus-mediated expression of defined transcription factor (TF) genes can effectively induce cellular reprogramming. However, sustained expression of the TFs often hinders pluripotent stem cell (PSC) differentiation into specific cell types, as each TF exerts its effect on PSCs for a defined period of time during differentiation. Here, we applied a bacterial type III secretion system (T3SS)-based protein delivery tool to directly translocate TFs in the form of protein into human PSCs. This transient protein delivery technique showed high delivery efficiency for hPSCs, and it avoids potential genetic alterations caused by the introduction of transgenes. In an established cardiomyocyte de novo differentiation procedure, five transcriptional factors, namely GATA4, MEF2C, TBX5, ESRRG and MESP1 (abbreviated as GMTEM), were translocated at various time points. By detecting the expression of cardiac marker genes (Nkx2.5 and cTnT), we found that GMTEM proteins delivered on mesoderm stage of the cardiomyocytes lineage differentiation significantly enhanced both the human ESC and iPSC differentiation into cardiomyocytes, while earlier or later delivery diminished the enhancing effect. Furthermore, all of the five factors were required to enhance the cardiac differentiation. This work provides a virus-free strategy of transient transcription factors delivery for directing human stem cell fate without jeopardizing genome integrity, thus safe for biomedical applications. [ABSTRACT FROM AUTHOR]

Published

2018

4. Enhanced Production of Recombinant Secretory Proteins in Pichia pastoris by Optimizing Kex2 P1’ site.

Author

Yang, Song, Kuang, Ye, Li, Hongbo, Liu, Yuehong, Hui, Xiaoyan, Li, Peng, Jiang, Zhiwu, Zhou, Yulai, Wang, Yu, Xu, Aimin, Li, Shiwu, Liu, Pentao, and Wu, Donghai

Subjects

RECOMBINANT proteins, PICHIA pastoris, GENE expression, AMINO acids, PROTEIN synthesis, AMINO acid residues

Abstract

Pichia pastoris is one of the most widely used expression systems for the production of recombinant secretory proteins. Its universal application is, however, somewhat hampered by its unpredictable yields for different heterologous proteins, which is now believed to be caused in part by their varied efficiencies to traffic through the host secretion machinery. The yeast endoprotease Kex2 removes the signal peptides from pre-proteins and releases the mature form of secreted proteins, thus, plays a pivotal role in the yeast secretory pathways. In this study, we found that the yields of many recombinant proteins were greatly influenced by Kex2 P1' site residues and the optimized P1’s amino acid residue could largely determine the final amount of secretory proteins synthesized and secreted. A further improvement of secretory yield was achieved by genomic integration of additional Kex2 copies, which again highlighted the importance of Kex2 cleavage to the production of recombinant secretory proteins in Pichia yeast. [ABSTRACT FROM AUTHOR]

Published

2013

5. High level expression of active recombinant human interleukin-3 in Pichia pastoris

Author

Li, Hongbo, Li, Na, Gao, Xuefei, Kong, Xiangping, Li, Shiwu, Xu, Aimin, Jin, Shouguang, and Wu, Donghai

Subjects

*GENE expression, *RECOMBINANT proteins, *PICHIA pastoris, *INTERLEUKIN-3, *HEMATOPOIETIC growth factors, *CELL differentiation, *ION exchange (Chemistry)

Abstract

Abstract: Interleukin-3 (IL-3) is a hematopoietic growth factor involved in the survival, proliferation and differentiation of multipotent hematopoietic cells. A DNA fragment containing the mature human IL-3 sequence was cloned into pPICZαA, generating a fusion protein with the alpha factor signal sequence in the N-terminus and 6×His as well as c-Myc tags in the C-terminus. The resulting plasmid was integrated into the genome of Pichia pastoris strain X-33. Recombinant yeast transformants with high-level rhIL-3 production were identified, secreting as much as 26mg/L rhIL-3 after 4days of induction by methanol in flask. The rhIL-3 was purified by Ni+-NTA affinity chromatography, followed by DEAE anion exchange, yielding over 95% highly purified rhIL-3 preparation at about 21mg/L. Mass spectrometry and MALDI-TOF-TOF analysis of the purified rIL-3 showed molecular weights of 18995.694Da and 22317.469Da, due to different degrees of N-linked glycosylation. The biological activity of the rhIL-3 proteins was confirmed by its ability to support ba/f3 cells proliferation and activate the ERK signaling pathways. The results demonstrate that the experimental procedure we have developed can produce a large amount of active recombinant human IL-3 from P. pastoris. [Copyright &y& Elsevier]

Published

2011

6. High level expression, purification and characterization of active fusion human C1q and tumor necrosis factor related protein 2 (hCTRP2) in Escherichia coli

Author

Li, Hongbo, Gao, Xuefei, Zhou, Yi, Li, Na, Ge, Caozuo, Hui, Xiaoyan, Wang, Yu, Xu, Aimin, Jin, Shouguang, and Wu, Donghai

Subjects

*GENE expression, *PROTEIN fractionation, *TUMOR necrosis factors, *ESCHERICHIA coli, *ADIPONECTIN, *BIOACTIVE compounds, *PICHIA pastoris, *RECOMBINANT proteins

Abstract

Abstract: C1q and tumor necrosis factor related proteins (CTRPs) are a family of adiponectin paralogues. Among them, CTRP2 is the only CTRP protein that has been shown to possess similar biological activities as adiponectin. To further explore the physiological roles of human CTRP2 and its mechanisms of action, hCTRP2 gene was expressed in Escherichia coli and Pichia pastoris, respectively. In the P. pastoris expression system, recombinant hCTRP2 could be secreted into the culture medium under induction condition, however, the resultant recombinant protein was highly unstable, resulting two main degradation products with molecular masses of approximately 20 and 26kDa, respectively. In the E. coli expression system, a large amount of soluble thioredoxin (Trx)-hCTRP2 fusion protein could be produced, which accounts about 42% of the total soluble bacterial proteins. The recombinant Trx-hCTRP2 fusion protein was purified to an approximately 95% purity using Ni-NTA affinity chromatography and Superdex G-75 column with a yield of about 15mg/l protein from 1l bacterial culture. The purified recombinant Trx-hCTRP2 was shown to be active under in vitro assay conditions. [Copyright &y& Elsevier]

Published

2011

7. Rosiglitazone promotes fatty acyl CoA accumulation and excessive glycogen storage in livers of mice without adiponectin

Author

Zhou, Mingyan, Xu, Aimin, Lam, Karen S.L., Tam, Paul K.H., Che, Chi-Ming, Chan, Lawrence, Lee, In-Kyu, Wu, Donghai, and Wang, Yu

Subjects

*ROSIGLITAZONE, *GLYCOGEN storage disease, *FATTY liver, *LABORATORY mice, *NON-alcoholic beverages, *MITOCHONDRIAL pathology, *GENE expression, *FATTY-acyl-CoA

Abstract

Background & Aims: The beneficial effects of rosiglitazone on non-alcoholic fatty liver disease (NAFLD) have been reported. Rosiglitazone treatment stimulates the production of adiponectin, an insulin-sensitizing adipokine with hepatoprotective functions. The present study aims to investigate the hepatic actions of rosiglitazone in mice without adiponectin. Methods: NAFLD was induced in wild type and adiponectin knockout (AKO) mice by high-fat diet feeding. After rosiglitazone treatment, mice were subjected to evaluations on systemic insulin sensitivity, lipid profiles, hepatic steatosis, and inflammation, as well as the expression and activity of key molecules involved in energy metabolism and mitochondrial functions. Results: Rosiglitazone treatment prevented hepatic inflammation and reduced the expression of pro-inflammatory cytokines in livers of wild type mice. In contrast, in livers of AKO mice, the same treatment induced severe hepatomegaly and microvesicular hepatosteatosis, and caused abnormal accumulation of fatty acyl CoA, glycogen, and their intermediate metabolites. Compared to wild type littermates, the anti-inflammatory and the mitochondria-stimulatory activity of rosiglitazone were largely attenuated in AKO mice. Replenishment with either adiponectin or uncoupling protein 2 (UCP2) significantly reduced fatty acyl CoA accumulation and increased mitochondrial activities in livers of rosiglitazone-treated AKO mice. In addition, adiponectin, but not UCP2, promoted the activation of glycogen synthase kinase 3beta (GSK3beta), a key molecule involved in regulating glycogen homeostasis. Conclusions: Rosiglitazone elicits its protective functions against NAFLD largely through the induction of adiponectin, which prevents mitochondria stresses by promoting GSK3beta activation and UCP2 upregulation, two pathways coordinating the glucose and lipid metabolism in liver. [ABSTRACT FROM AUTHOR]

Published

2010

8. Identification and preliminary functional analysis of alternative splicing of Siah1 in Xenopus laevis

Author

Wen, Luan, Liu, Jiantao, Chen, Yonglong, and Wu, Donghai

Subjects

*GENETIC engineering, *XENOPUS laevis, *PROTEINS, *FUNCTIONAL analysis, *DROSOPHILA genetics, *GENE expression, *AMINO acids

Abstract

Abstract: Siah proteins are vertebrate homologs of the Drosophila ‘seven in absentia’ gene. In this study, we characterized two splicing forms, Siah1a and Siah1b, of the Xenopus seven in absentia homolog 1 gene (Siah1). Overexpression of xSiah1a led to severe suppression of embryo cleavage, while that of xSiah1b was not effective even at a high dose. Competition analysis demonstrated that co-expression of xSiah1a and 1b generated the same phenotype as overexpression of xSiah1a alone, suggesting that xSiah1b does not interfere with the function of xSiah1a. Since xSiah1b has an additional 31 amino acids in the N-terminus compared to xSiah1a, progressive truncation of xSiah1b from the N-terminus showed that inability of xSiah1b to affect embryo cleavage was associated with the length of the N-terminal extension of extra amino acids. The possible implication of this finding is discussed. [Copyright &y& Elsevier]

Published

2010

9. High level expression and purification of active recombinant human interleukin-8 in Pichia pastoris

Author

Li, Hongbo, Wang, Dongye, Xu, Aimin, Li, Shiwu, Jin, Shouguang, and Wu, Donghai

Subjects

*GENE expression, *PROTEIN fractionation, *INTERLEUKIN-8, *NEOVASCULARIZATION, *PICHIA pastoris, *RECOMBINANT proteins

Abstract

Abstract: Human interleukin-8 (hIL-8) is a member of interleukin family which functions as a chemotactic factor as well as an angiogenesis mediator. Previously, a study reported that hIL-8 could be purified from inclusion bodies using a prokaryotic expression system, however, the required re-naturation step limits the recovery of fully active protein. In this study, soluble recombinant hIL-8 was expressed as a secreted protein at high level in Pichia pastoris under the control of AOX1 (alcohol oxidase 1) promoter. A simple purification strategy was established to recover rhIL-8 from the fermentation supernatant. The process includes precipitation with 80% saturation ammonium sulfate and CM Sepharose ion exchange chromatography, yielding 30mg/L purified rhIL-8 at over 95% purity. The obtained rhIL-8 displays high specific activity, stimulating the migration of mouse neutrophils at concentrations as low as 0.25ng/mL. Our results demonstrate that P. pastoris expression system is an efficient tool for large-scale manufacture of active recombinant hIL-8 for various applications. [Copyright &y& Elsevier]

Published

2009

10. Up-regulation of a non-kinase activity isoform of Ca2+/calmodulin-dependent protein kinase kinase beta1 (CaMKKβ1) in hibernating bat brain

Author

Yuan, Lihong, Chen, Jinping, Lin, Benfu, Liang, Bing, Zhang, Shuyi, and Wu, Donghai

Subjects

*HIBERNATION, *LOW temperatures, *FOOD supply, *GENE expression, *PHOSPHORYLATION

Abstract

Abstract: Hibernation is an adaptive strategy that is utilized by some animals to survive the harsh environments of low temperature and food scarce. Hibernators, however, can survive in frequent and dramatic fluctuation of body temperature and blood flow causing by periodic arousals during hibernation without brain insult, and this indicates that it must have some unique adaptive aspects of hibernation physiology. To find out the up-regulated genes of bat brain during hibernation and explore the brain function adaptive mechanism of bat, the suppression subtractive hybridization (SSH) library was constructed from the brain tissue of greater horseshoe bats. Dot blot screening was carried out and the up-regulated genes in hibernating state were obtained. Then RT-PCR and RQ-PCR were performed to test the expression patterns of selected cDNAs. Here we first show that the functional and non-functional isoforms of bat CaMKKβ1 display distinct expression patterns between hibernating and active states. The up-regulation of non-functional form of CaMKKβ1 may represent a new neuroprotective strategy adopted by bats or even other hibernators to avoid the CNS damage during hibernation. Our results showed that bat CaMKKβ1 gene has four transcript isoforms and these transcript variants differ primarily in exons b and d, which are 129 bp and 43 bp respectively. Statistical analyses indicated that these isoforms display distinct expression patterns at different states, in which only isoform 3, the non-functional form, increased 300% at hibernating state. These results suggest that distinct expression patterns of transcript isoforms of a gene, which have different activity, may represent a new potential adaptive mechanism in hibernation, except for the simple up-regulation of selected genes/proteins and the reversible protein phosphorylation. [Copyright &y& Elsevier]

Published

2007

11. The truA gene of Pseudomonas aeruginosa is required for the expression of type III secretory genes.

Author

Ahn, Kyung-Seop, Ha, Unhwan, Jia, Jinghua, Wu, Donghai, and Jin, Shouguang

Subjects

*PSEUDOMONAS aeruginosa, *GENE expression, *GENES, *GENETIC mutation, *PROTEINS, *TRANSFER RNA

Abstract

Invasive strains of Pseudomonas aeruginosa can cause rapid host cell apoptosis by injecting the type III effector molecule ExoS. A transposon insertional mutant bank of P. aeruginosa was screened to identify P. aeruginosa genes that contribute to the ability of the bacteria to trigger host cell apoptosis. Several isolated mutants had disruptions in the fimV gene. A fimV mutant was unable to induce the expression of exoS, exoT and exsA genes under type III inducing conditions, thus exhibiting a defect in type III protein secretion. Furthermore, this mutant was defective in twitching motility, although type IV pili were present on the bacterial surface. Complementation by a fimV-containing cosmid clone restored both phenotypes to the wild-type levels. However, expression of the type III genes in the fimV mutant was not restored by the introduction of a fimV gene alone, although it restored the twitching motility. A gene downstream of fimV, encoding a tRNA pseudouridine synthase (truA) homologue, was able to complement the type III gene expression defect of the fimV mutant. Thus firnV and truA form an operon and fimV mutation has a polar effect on truA. Indeed, a truA mutant is defective in type III gene expression while its twitching motility is unaffected, and a truA clone is able to complement the type III secretion defect. Pseudouridination of tRNAs is important for tRNA structure, thereby improving the fidelity of protein synthesis and helping to maintain the proper reading frame; thus the results imply that truA controls tRNAs that are critical for the translation of type III genes or their regulators. [ABSTRACT FROM AUTHOR]

Published

2004