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Dive into the research topics where Chuanpeng Liu is active.

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Featured researches published by Chuanpeng Liu.


The International Journal of Biochemistry & Cell Biology | 2010

PPIase domain of trigger factor acts as auxiliary chaperone site to assist the folding of protein substrates bound to the crevice of trigger factor

Chuanpeng Liu; Qiming Zhou; Dongjie Fan; Jun-Mei Zhou

Trigger factor (TF) is the first chaperone encountered by nascent chains in bacteria, which consists of two modules: peptidyl-prolyl-cis/trans-isomerase (PPIase) domain and a crevice built by both N- and C-terminal domains. While the crevice is suggested to provide a protective space over the peptide exit site of ribosome for nascent polypeptides to fold, it remains unclear whether PPIase domain is directly involved in assisting protein folding. Here, we introduced structural change into different regions of TF, and investigated their influence on the chaperone function of TF in assisting the folding of various substrate proteins, including oligomeric glyceraldehyde-3-phosphate dehydrogenase (GAPDH) and monomeric carbonic anhydrase II (CA II) and lysozyme. Results showed that structural disturbances by site-specific mutations in the PPIase active site or by deletion of the PPIase domain from TF affected the chaperone activity of TF toward CA II and GAPDH but had no effect on TF-assisted lysozyme refolding, suggesting PPIase domain is involved in assisting the folding of substrates larger than lysozyme. Mutants with the structural disturbances in the crevice totally lost the chaperone activity toward all the substrates we used in this investigation. These results provide further evidence to confirm that the crevice is the major chaperone site of TF, and the hydrophobic pocket in PPIase domain acts as an auxiliary site to assist the folding of substrate proteins bound to the crevice in a substrate-dependent manner, which is beneficial for TF to provide appropriate assistance for protein folding by changing protective space and binding affinity.


World Journal of Microbiology & Biotechnology | 2010

A method for generating precise gene deletions and insertions in Escherichia coli

Qiming Zhou; Dongjie Fan; Jiang-Bi Xie; Chuanpeng Liu; Jun-Mei Zhou

A simple and general method for disrupting chromosomal genes and introducing insertions is described. This procedure involves eliminating wild-type bacterial genes and introducing mutant alleles or other insertions at the original locus of the wild-type gene. To demonstrate the utility of this approach, the tig gene of Escherichia coli was replaced by homologous recombination with a cassette containing the chloramphenicol resistance gene and the sacB gene. The cassette was then removed and the tig mutant alleles were moved into the native tig location. Sequencing and Western blotting results demonstrated that insertions or deletions can be introduced precisely in E. coli using our approach. Our system does not require extra in vitro manipulations such as restriction digestion or ligation, and does not require use of specific plasmids or strains which are used to prevent false positive transformants caused by template plasmid transformation. This technique can be used widely in bacterial genome analysis.


BMC Microbiology | 2015

Distribution patterns of haplotypes for symbionts from Umbilicaria esculenta and U. muehlenbergii reflect the importance of reproductive strategy in shaping population genetic structure

Shunan Cao; Fang Zhang; Chuanpeng Liu; Zhihua Hao; Yuan Tian; Lingxiang Zhu; Qiming Zhou

BackgroundThe diversity of lichen fungal components and their photosynthetic partners reflects both ecological and evolutionary factors. In present study, molecular investigations of the internal transcribed spacer of the nuclear ribosomal DNA (ITS nrDNA) region were conducted to analyze the genetic diversity of Umbilicaria esculenta and U. muehlenbergii together with their associated green algae.ResultIt was here demonstrated that the reproductive strategy is a principal reason for fungal selectivity to algae. U. muehlenbergii, which disperses via sexual spores, exhibits lower selectivity to its photosynthetic partners than U. esculenta, which has a vegetative reproductive strategy. The difference of genotypic diversity (both fungal and algal) between these two Umbilicaria species is low, although their nucleotide diversity can vary greatly.ConclusionsThe present study illustrates that lichen-forming fungi with sexual reproductive strategies are less selective with respect to their photobionts; and reveals that both sexual and vegetative reproduction allow lichens to generate similar amounts of diversity to adapt to the environments. The current study will be helpful for elucidating how lichens with different reproductive strategies adapt to changing environments.


Polar Research | 2017

Patterns of fungal–algal symbiont association in Usnea aurantiaco-atra reveal the succession of lichen–moss communities in Fildes Peninsula, Antarctica

Shunan Cao; Fang Peng; Hongyuan Zheng; Feng Wang; Chuanpeng Liu; Qiming Zhou

ABSTRACT Usnea aurantiaco-atra is the most widespread flora in Fildes Peninsula. There are two growth types of U. aurantiaco-atra: the erect form on rocks and the prostrate form associated with mosses. Phylogenetic analysis showed that individuals of the two growth forms share genotypes. Moreover, haploid disequilibrium testing indicated no significant genetic difference for the two growth forms when fungal and algal internal transcribed spacer rDNA were treated as two alleles of one lichen individual. The two growth forms of U. aurantiaco-atra appear to reflect different stages of lichen–moss community succession. A mode is proposed for demonstrating the occurrence of this succession.


Microbiological Research | 2016

Large-scale gene expression profiling reveals physiological response to deletion of chaperone dnaKJ in Escherichia coli

Dongjie Fan; Chuanpeng Liu; Lushan Liu; Lingxiang Zhu; Fang Peng; Qiming Zhou

Chaperone DnaK and its co-chaperone DnaJ plays various essential roles such as in assisting in the folding of nascent peptides, preventing protein aggregation and maintaining cellular protein homeostasis. Global transcriptional changes in vivo associated with deletion of dnaKJ were monitored using DNA microarray to elucidate the role of DnaKJ at the transcriptional level. Microarray profiling and bioinformatics analysis revealed that a few chaperone and protease genes, stress-related genes and genes involved in the tricarboxylic acid cycle and oxidative phosphorylation were up-regulated, whereas various transporter genes, pentose phosphate pathway and transcriptional regulation related genes were down-regulated. This study is the first to systematically analyze the alterations at the transcriptional level in vivo in deletion of dnaKJ. Fatty acid methyl esters analysis indicated that the amount of unsaturated fatty acid sharply increased and subcellular location prediction analysis showed a marked decrease in transcription of inner-membrane protein genes, which might have triggered the development of aberrant cell shape and susceptibility for some antibiotics in the ΔdnaKJ strain.


Science China-life Sciences | 2012

A glimpse of enzymology within the idea of systems

Chuanpeng Liu; Dongjie Fan; Yi Shi; Qiming Zhou

School of Life Science and Technology, Harbin Institute of Technology, Harbin 150080, China; National Institute for Communicable Disease Control and Prevention, Chinese Center for Disease Control and Prevention, Beijing 102206, China; Center for Stem Cell and Regenerative Medicine, Shanghai Advanced Research Institute, Chinese Academy of Sciences, Shanghai 201203, China; State Key Laboratory of Mycology, Institute of Microbiology, Chinese Academy of Sciences, Beijing 100101, China


The FASEB Journal | 2018

Exploring the roles of substrate-binding surface of the chaperone site in the chaperone activity of trigger factor

Dongjie Fan; Shunan Cao; Qiming Zhou; You Zhang; Lei Yue; Chang Han; Bo Yang; Yu Wang; Zhuo Ma; Lingxiang Zhu; Chuanpeng Liu

Trigger factor (TF) is a key component of the prokaryotic chaperone network, which is involved in many basic cellular processes, such as protein folding, protein trafficking, and ribosome assembly. The major chaperone site of TF has a cradle‐like structure in which protein substrate may fold without interference from other proteins. Here, we investigated in vivo and in vitro the roles of hydrophobic and charged patches on the edge and interior of cradle during TF‐assisted protein folding. Our results showed that most of the surface of the cradle was involved in TF‐assisted protein folding, which was larger than found in early studies. Although the inner surface of cradle was mostly hydrophobic, both hydrophobic and electrostatic patches were indispensable for TF to facilitate correct protein folding. However, hydrophobic patches were more important for the antiaggregation activity of TF. Furthermore, it was found that the patches on the surface of cradle were involved in TF‐assisted protein folding in a spatial and temporal order. These results suggest that the folding‐favorable interface between the cradle and substrate was dynamic during TF‐assisted protein folding, which enabled TF to be involved in the folding of substrate in an aggressive manner rather than acting as a classic holdase.—Fan, D., Cao, S., Zhou, Q., Zhang, Y., Yue, L., Han, C., Yang, B., Wang, Y., Ma, Z., Zhu, L., Liu, C. Exploring the roles of substrate‐binding surface of the chaperone site in the chaperone activity of trigger factor. FASEB J. 32, 6655–6665 (2018). www.fasebj.org


PhytoKeys | 2018

Coccomyxa antarctica sp. nov. from the Antarctic lichen Usnea aurantiacoatra

Shunan Cao; Fang Zhang; Hongyuan Zheng; Chuanpeng Liu; Fang Peng; Qiming Zhou

Abstract The single celled green alga Coccomyxa antarctica Shunan Cao & Qiming Zhou, sp. nov. was isolated from the Antarctic torrential lichen Usnea aurantiacoatra (Jacq.) Bory. It is described and illustrated based on a comprehensive study of its morphology, ultrastructure, ecology and phylogeny. C. antarctica is a lichenicolous alga which has elongated cells and contains a parietal chloroplast as observed under the microscope. C. antarctica is clearly different from other species by phylogenetic analysis (ITS rDNA and SSU rDNA sequences), also it differs from its phylogenetic closely species C. viridis by its larger cell size.


Journal of Cellular Biochemistry | 2017

Global Analysis of the Impact of Deleting Trigger Factor on the Transcriptome Profile of Escherichia coli.

Dongjie Fan; Lushan Liu; Lingxiang Zhu; Fang Peng; Qiming Zhou; Chuanpeng Liu

Trigger factor (TF) is a key component of prokaryotic chaperone network, which is involved various basic cellular processes such as nascent peptide folding, protein trafficking, ribosome assembly. To better understanding the physiological roles of TF, global transcriptome profiles of a variety of TF deletion mutant strains of Escherichia coli were determined. We found that deletion of the tig gene, encoding TF, led to a dramatic alteration of transcriptome profile, not only affecting the gene expression of members of the chaperone network, but also changing the levels of quite a few RNAs related to metabolism and other cellular processes. Further studies showed that this alteration was only partially recovered by knockin of TF domain‐deletion mutants into the endogenous tig locus, indicating that structural integrity is crucial for the biological function of TF. Finally, by combining the transcriptome and phenotype results, a physiological mechanism underlying the impact of TF deletion on the transcriptome profile was proposed. J. Cell. Biochem. 118: 141–153, 2017.


Microbiological Research | 2016

Functional characterization of the Helicobacter pylori chaperone protein HP0795

Dongjie Fan; Qiming Zhou; Chuanpeng Liu; Jianzhong Zhang

Trigger factor (TF) is one of the multiple bacterial chaperone proteins interacting with nascent peptides and facilitating their folding in bacteria. While TF is well-characterized in E. coli, HP0795, a TF-like homologue gene identified earlier in the pathogenic Helicobacter pylori (H. pylori), has not been studied biochemically to date. To characterize its function as a chaperone, we performed 3D-modeling, cross-linking and in vitro enzyme assays to HP0795 in vitro. Our results show that HP0795 possesses peptidyl prolyl cis-trans isomerase activity and exhibits a dimeric structure in solution. In addition, stable expression of HP0795 in a series of well-characterized E. coli chaperone-deficient strains rescued the growth defects in these mutants. Furthermore, we showed that the presence of HP0795 greatly reduced protein aggregation caused by deficiencies of chaperones in these strains. In contrast to other chaperone genes in H. pylori, gene expression of HP0795 displays little induction under acidic pH conditions. Together, our results suggest that HP0795 is a constitutively expressed TF-like protein of the prokaryotic chaperone family that may not play a major role in acid response. Given the pathogenic properties of H. pylori, our insights might provide new avenues for potential future medical intervention for H. pylori-related conditions.

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Qiming Zhou

Harbin Institute of Technology

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Dongjie Fan

Chinese Center for Disease Control and Prevention

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Shunan Cao

Polar Research Institute of China

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Fang Zhang

Polar Research Institute of China

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Lingxiang Zhu

Beijing Institute of Genomics

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Jun-Mei Zhou

Chinese Academy of Sciences

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Lushan Liu

China Rehabilitation Research Center

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