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Dive into the research topics where Yundong Sun is active.

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Featured researches published by Yundong Sun.


Journal of Microbiology | 2009

Helicobacter pylori proteins response to nitric oxide stress

Wei Qu; Yabin Zhou; Chunhong Shao; Yundong Sun; Qunye Zhang; Chunyan Chen; Jihui Jia

Helicobacter pylori is a highly pathogenic microorganism with various strategies to evade human immune responses. Nitric oxide (NO) and reactive nitrogen species (RNS) generated via nitric oxide synthase pathway are important effectors during the innate immune response. However, the mechanisms of H. pylori to survive the nitrosative stress are not clear. Here the proteomic approach has been used to define the adaptive response of H. pylori to nitrosative stress. Proteomic analysis showed that 38 protein spots were regulated by NO donor, sodium nitroprusside (SNP). These proteins were involved in protein processing, anti-oxidation, general stress response, and virulence, as well as some unknown functions. Particularly, some of them were participated in iron metabolism, potentially under the control of ferric uptake regulator (Fur). Real time PCR revealed that fur was induced under nitrosative stress, consistent with our deduction. One stress-related protein up-regulated under nitrosative conditions was thioredoxin reductase (TrxR). Inactiva-tion of fur or trxR can lead to increased susceptivity to nitrosative stress respectively. These studies described the adaptive response of H. pylori to nitric oxide stress, and analyzed the relevant role of Fur regulon and TrxR in nitrosative stress management.


Journal of Medical Microbiology | 2008

Helicobacter pylori protein response to human bile stress

Chunhong Shao; Qunye Zhang; Yundong Sun; Zhifang Liu; Jiping Zeng; Yabin Zhou; Xiuping Yu; Jihui Jia

The ability of Helicobacter pylori to tolerate bile is likely to be important for its colonization and survival in the gastrointestinal tract of humans. As bile can be acidified after reflux into the low pH of the human stomach, the inhibitory effect of fresh human bile with normal appearance on H. pylori before and after acidification was tested first. The results showed that acidification of bile attenuated its inhibitory activity towards H. pylori. Next, the protein profiles of H. pylori under human bile and acidified bile stress were obtained by two-dimensional electrophoresis. Protein spots with differential expression were identified using tandem matrix-assisted laser desorption/ionization time-of-flight mass spectrometry. The results showed that the changes in proteomic profiles under bile and acidified bile stress were similar when compared with that of normal H. pylori. Expression of 28 proteins was found to be modulated, with the majority being induced during bile or acidified bile exposure. These proteins included molecular chaperones, proteins involved in iron storage, chemotaxis protein, enzymes related to energy metabolism and flagellar protein. These results indicate that H. pylori responds to bile and acidified bile stress through multiple mechanisms involving many signalling pathways.


Journal of Microbiology | 2008

The changes of proteomes components of Helicobacter pylori in response to acid stress without urea

Chunhong Shao; Qunye Zhang; Wei Tang; Wei Qu; Yabin Zhou; Yundong Sun; Han Yu; Jihui Jia

Acid stress is the most obvious challenge Helicobacter pylori encounters in human stomach. The urease system is the basic process used to maintain periplasmic and cytoplasmic pH near neutrality when H. pylori is exposed to acidic condition. However, since the urea concentration in gastric juice is approximately 1 mM, considered possibly insufficient to ensure the survival of H. pylori, it is postulated that additional mechanisms of pH homeostasis may contribute to the acid adaptation in H. pylori. In order to identify the acid-related proteins other than the urease system we have compared the proteome profiles of H. pylori strain 26695 exposed to different levels of external pH (7.4, 6.0, 5.0, 4.0, 3.0, and 2.0) for 30 min in the absence of urea using 2-DE. Differentially expressed proteins were identified by MALDI-TOF-TOF-MS analysis, which turned out to be 36 different proteins. The functions of these proteins included ammonia production, molecular chaperones, energy metabolism, cell envelope, response regulator and some proteins with unknown function. SOM analysis indicated that H. pylori responds to acid stress through multi-mechanisms involving many proteins, which depend on the levels of acidity the cells encounter.


Laser Physics | 2009

Analysis of a laser-diode end-pumped passively Q-switched Nd:GdVO4 laser with V3+:YAG saturable absorber

Jinlong Ma; Y. Li; Yundong Sun; H.J. Qi; R.J. Lan; Xueyuan Hou

By considering both the transversal and longitudinal Gaussian spatial distribution of the intracavity photon density, a couple of rate equations describing a laser-diode end-pumped passively Q-switched Nd:GdVO4 laser with V3+:YAG saturable absorber have been proposed. Solving these space-dependent rate equations numerically, we obtain the dependences of pulse width, pulse repetition rate, single-pulse energy and peak power on pump power. In the experiment, a laser-diode end-pumped Nd:GdVO4 laser passively Q-switched by a V3+:YAG saturable absorber has been realized, and the experimental results are consistent with the theoretical calculations.


Journal of Microbiology | 2011

Identification of S-nitrosylation of proteins of Helicobacter pylori in response to nitric oxide stress.

Wei Qu; Yabin Zhou; Yundong Sun; Ming Fang; Han Yu; Wenjuan Li; Zhifang Liu; Jiping Zeng; Chunyan Chen; Chengjiang Gao; Jihui Jia

Innate and adaptive immune responses are activated in humans when Helicobacter pylori invades the gastric mucosa. Nitric oxide (NO) and reactive nitrogen species are important immune effectors, which can exert their functions through oxidation and S-nitrosylation of proteins. S-nitrosoglutathione and sodium nitroprus-side were used as NO donors and H. pylori cells were incubated with these compounds to analyze the inhibitory effect of NO. The suppressing effect of NO on H. pylori has been shown in vitro. Furthermore, the proteins modified by S-nitrosylation in H. pylori were identified through the biotin switch method in association with matrix-assisted laser desorption ionization/time-of-flight tandem mass spectrometry (MALDI-TOF-MS/MS). Five S-nitrosylated proteins identified were a chaperone and heat-shock protein (GroEL), alkyl hydroperoxide reductase (TsaA), urease alpha subunit (UreA), HP0721, and HP0129. Importantly, S-nitrosylation of TsaA and UreA were confirmed using purified recombinant proteins. Considering the importance of these enzymes in antioxidant defenses, adherence, and colonization, NO may exert its antibacterial actions by targeting enzymes through S-nitrosylation. Identification of protein S-nitrosylation may contribute to an understanding of the antibacterial actions of NO. Our findings provide an insight into potential targets for the development of novel therapeutic agents against H. pylori infection.


Laser Physics | 2010

Doubly passively Q-switched laser with V3+:YAG and Co:LMA saturable absorbers

Y. Li; S. Zhao; Yundong Sun; H.J. Qi

By using both V3+:YAG and Co:LMA saturable absorbers, a doubly passively Q-switched laser is realized for the first time. The shorter pulse with the higher peak power is generated in comparison to the singly passively Q-switched laser with V3+:YAG or Co:LMA saturable absorber. The experimental results shows that it is possible to obtain a shorter pulse with the higher peak power in a doubly passively Q-switched laser.


Current Microbiology | 2012

Analysis of Aztreonam-Inducing Proteome Changes in Nondividing Filamentous Helicobacter pylori

Chunhong Shao; Yabin Zhou; Yundong Sun; Hongyan Wang; Wei Qu; Han Yu; Chunyan Chen; Jihui Jia

When stressed, bacteria can enter various nondividing states. In the present study, nondividing filamentous form in Helicobacter pylori was induced by a β-lactam antibiotic, aztreonam. In order to find possible cell division checkpoints in H. pylori, 2-DE was used to compare the proteomic profile of nondividing filamentous H. pylori with its spiral form. In total, 21 proteins involved in various cellular processes showed differential expression. One protein induced by aztreonam was a cell division inhibitor (minD), related to cell division. We then constructed the deletion mutant of minD in H. pylori 26695. Scanning electron microscope observation showed that the deletion of this protein provoked some bacteria to change into a short rod-shape and the viability of the mutant is lower than that of the wild type. Moreover, sequence comparison showed that minD of H. pylori and that of Escherichia coli share 50xa0% amino acid identity. This suggested that this protein possibly plays the similar part in H. pylori as in E. coli.


Laser Physics | 2010

Doubly passively Q-switched and mode-locked laser with V3+:YAG and Co:LMA saturable absorbers

Y. Li; S. Zhao; Yundong Sun; H.J. Qi

By using both V3+:YAG and Co:LMA saturable absorbers, an xenon-lamp-pumped doubly passively Q-switched and mode-locked (QML) Nd:YAG laser at 1.3 μm in a straight cavity is realized for the first time. The modulation depth of QML pulse has nearly reached 100%. The experimental results shows that the doubly passively Q-switched and mode-locked (QML) laser can generate shorter Q-switch envelope pulse with higher average peak power in comparison to the singly passively QML laser with V3+:YAG or Co:LMA saturable absorber.


Laser Physics | 2010

Passively Q-switched and mode-locked 1.3 μm Nd:YAG laser with Co:LMA saturable absorber

Y. Li; S. Zhao; Yundong Sun; H.J. Qi; G.H. Zhang

An xenon-lamp-pumped passively Q-switched and mode-locked (QML) Nd:YAG laser with Co:LMA saturable absorber at 1.3 μm is realized in a straight cavity. The modulation depth of mode locking pulse has reached 100%. The pulse energy and the pulse width of QML laser have been measured. The pulse width of the mode-locking laser is estamated to be 940 ps.


Antimicrobial Agents and Chemotherapy | 2017

The Bifunctional Enzyme SpoT Is Involved in the Clarithromycin Tolerance of Helicobacter pylori by Upregulating the Transporters HP0939, HP1017, HP0497, and HP0471

Xiwen Geng; Wen Li; Zhenghong Chen; Sizhe Gao; Wei Hong; Xiaoran Ge; Guihua Hou; Zhekai Hu; Yabin Zhou; Beini Zeng; Wenjuan Li; Jihui Jia; Yundong Sun

ABSTRACT Clarithromycin (CLA) is a commonly recommended drug for Helicobacter pylori eradication. However, the prevalence of CLA-resistant H. pylori is increasing. Although point mutations in the 23S rRNA are key factors for CLA resistance, other factors, including efflux pumps and regulation genes, are also involved in the resistance of H. pylori to CLA. Guanosine 3′-diphosphate 5′-triphosphate and guanosine 3′,5′-bispyrophosphate [(p)ppGpp)], which are synthesized by the bifunctional enzyme SpoT in H. pylori, play an important role for some bacteria to adapt to antibiotic pressure. Nevertheless, no related research involving H. pylori has been reported. In addition, transporters have been found to be related to bacterial drug resistance. Therefore, this study investigated the function of SpoT in H. pylori resistance to CLA by examining the shifts in the expression of transporters and explored the role of transporters in the CLA resistance of H. pylori. A ΔspoT strain was constructed in this study, and it was shown that SpoT is involved in H. pylori tolerance of CLA by upregulating the transporters HP0939, HP1017, HP0497, and HP0471. This was assessed using a series of molecular and biochemical experiments and a cDNA microarray. Additionally, the knockout of genes hp0939, hp0471, and hp0497 in the resistant strains caused a reduction or loss (the latter in the Δhp0497 strain) of resistance to CLA. Furthermore, the average expression levels of these four transporters in clinical CLA-resistant strains were considerably higher than those in clinical CLA-sensitive strains. Taken together, our results revealed a novel molecular mechanism of H. pylori adaption to CLA stress.

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Han Yu

Shandong University

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Wei Qu

Shandong University

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