Your search keyword '"Cystatin C biosynthesis"' showing total 26 results

1. Expression, purification and identification of isotope-labeled recombinant cystatin C protein in Escheichia coli intended for absolute quantification using isotope dilution mass spectrometry.

Author

Zhang Q, Cai Z, Lin H, Han L, Yan J, Wang J, Ke P, Zhuang J, and Huang X

Subjects

Humans, Mass Spectrometry, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins genetics, Cystatin C biosynthesis, Cystatin C genetics, Escherichia coli chemistry, Escherichia coli genetics, Escherichia coli metabolism, Gene Expression, Nitrogen Isotopes chemistry

Abstract

Isotope-labeled proteins are expected to be used as internal standard proteins in the field of protein quantification by isotope dilution mass spectrometry (ID/MS). To achieve the absolute quantification of Cystatin C (Cys C) based on ID/MS, we aims to obtain 15 N isotope-labeled recombinant Cys C ( 15 N-Cys C) protein. Firstly, the Cys C gene was optimized based on the preferred codons of Escherichia coli, and inserted into the pET-28a(+) expression plasmid. Then, the plasmid was transformed into TOP10 and BL21 strains, and 15 N-Cys C was expressed in M9 medium using 15 N as the only nitrogen source. 15 N-Cys C was detected by SDS-PAGE, protein immunoblotting and matrix-assisted laser desorption/ionization-time of flight mass spectrometry (MALDI-TOF MS). The characteristic peptides obtained from 15 N-Cys C were analyzed by a Q Exactive Plus MS system. Results showed that 53.06% of the codons were optimized. The codon adaptation index of the Cys C genes increased from 0.31 to 0.95, and the GC content was adjusted from 64.85% to 54.88%. The purity of 15 N-Cys C was higher than 95%. MALDI-TOF MS analysis showed that the m/z of 15 N-Cys C had changed from 13 449 to 14 850. The characteristic peptides showed that 619.79 m/z (M+2H) 2+ was the parent ion of 15 N-Cys C and that the secondary ions of 15 N-labeled peptides from y +5 to y +9 were 616.27 m/z, 716.33 m/z, 788.39 m/z, 936.43 m/z, and 1052.46 m/z, respectively. In conclusion, we successfully expressed, purified and identified of 15 N-Cys C protein in Escheichia coli intended for absolute quantification using ID/MS., (Copyright © 2020 Elsevier Inc. All rights reserved.)

Published

2021

2. Cystatin C improves blood-brain barrier integrity after ischemic brain injury in mice.

Author

Yang B, Xu J, Chang L, Miao Z, Heang D, Pu Y, Zhou X, Zhang L, and Xie H

Subjects

Animals, Blood-Brain Barrier drug effects, Blood-Brain Barrier pathology, Brain Injuries drug therapy, Brain Injuries pathology, Brain Ischemia drug therapy, Brain Ischemia pathology, Infusions, Intraventricular, Male, Mice, Mice, Inbred ICR, Blood-Brain Barrier metabolism, Brain Injuries metabolism, Brain Ischemia metabolism, Cystatin C administration & dosage, Cystatin C biosynthesis

Abstract

Cystatin C, a well-established biomarker of renal function, has been associated with a protective effect against stroke. However, the potential neuroprotective mechanism of cystatin C in ischemic brain injury remains unclear. Our study hypothesized that cystatin C can ameliorate blood-brain barrier (BBB) disruption by up-regulating caveolin-1 expression, thereby improving neurological outcomes in cerebral ischemic injury. Western blotting, immunohistochemistry, immunofluorescence staining, and immunoprecipitation were performed to investigate target proteins. Evans Blue and gelatin zymography were used to examine the effect of cystatin C on BBB disruption. Plasmid and small interfering RNA transfection was used to observe alterations in caveolin-1 and occludin expression induced by changes in cystatin C expression. Intriguingly, our study showed that the expression of both cystatin C and caveolin-1 was increased in middle cerebral artery occlusion-injured mice, and pretreatment with exogenous cystatin C significantly increased caveolin-1 expression, reduced Evans Blue leakage in the injured brain region, and decreased the enzymatic activity of matrix metallopeptidase-9. Meanwhile, our study also showed that the over-expression of cystatin C greatly enhanced caveolin-1 expression, which later increased occludin expression in oxygen-glucose deprivation-exposed brain microvascular endothelial cells. The knockdown of cystatin C induced the opposite outcomes. These experimental results indicate a positive role for cystatin C in the regulation of caveolin-1 and occludin expression in cerebral ischemic injury. Taken together, these data unveil a new mechanism of the regulation of caveolin-1 expression by cystatin C in the maintenance of BBB integrity after ischemic brain injury and provide new clues for the identification of potential therapeutic strategies for stroke., (© 2019 International Society for Neurochemistry.)

Published

2020

3. Cystatin C prevents neuronal loss and behavioral deficits via the endosomal pathway in a mouse model of down syndrome.

Author

Kaur G, Gauthier SA, Perez-Gonzalez R, Pawlik M, Singh AB, Cosby B, Mohan PS, Smiley JF, and Levy E

Subjects

Animals, Cystatin C genetics, Down Syndrome genetics, Endosomes genetics, Female, Male, Mice, Mice, Inbred C57BL, Mice, Transgenic, Phosphatidylinositol 3-Kinases genetics, Phosphatidylinositol 3-Kinases metabolism, Cystatin C biosynthesis, Disease Models, Animal, Down Syndrome metabolism, Endosomes metabolism, Signal Transduction physiology

Abstract

Cystatin C (CysC) plays diverse protective roles under conditions of neuronal challenge. We investigated whether CysC protects from trisomy-induced pathologies in a mouse model of Down syndrome (DS), the most common cause of developmental cognitive and behavioral impairments in humans. We have previously shown that the segmental trisomy mouse model, Ts[Rb(12.1716)]2Cje (Ts2) has DS-like neuronal and behavioral deficiencies. The current study reveals that transgene-mediated low levels of human CysC overexpression has a preventive effect on numerous neuropathologies in the brains of Ts2 mice, including reducing early and late endosome enlargement in cortical neurons and decreasing loss of basal forebrain cholinergic neurons (BFCNs). Consistent with these cellular benefits, behavioral dysfunctions were also prevented, including deficits in nesting behavior and spatial memory. We determined that the CysC-induced neuroprotective mechanism involves activation of the phosphotidylinositol kinase (PI3K)/AKT pathway. Activating this pathway leads to enhanced clearance of accumulated endosomal substrates, protecting cells from DS-mediated dysfunctions in the endosomal system and, for BFCNs, from neurodegeneration. Our findings suggest that modulation of the PI3/AKT pathway offers novel therapeutic interventions for patients with DS., (Copyright © 2018 Elsevier Inc. All rights reserved.)

Published

2018

4. Cystatin C Expression is Promoted by VEGFA Blocking, With Inhibitory Effects on Endothelial Cell Angiogenic Functions Including Proliferation, Migration, and Chorioallantoic Membrane Angiogenesis.

Author

Li Z, Wang S, Huo X, Yu H, Lu J, Zhang S, Li X, Cao Q, Li C, Guo M, Lv J, Du X, and Chen Z

Subjects

Animals, Cell Movement, Cell Proliferation, Gerbillinae, Neovascularization, Pathologic, Neovascularization, Physiologic, Chorioallantoic Membrane blood supply, Cystatin C biosynthesis, Endothelial Cells physiology, Vascular Endothelial Growth Factor A physiology

Abstract

Background Vascular development, including vasculogenesis and angiogenesis, is involved in many diseases. Cystatin C ( CST 3) is a commonly used marker of renal dysfunction, and we have previously reported that its expression level is associated with variations in the gerbil circle of Willis. Thus, we hypothesized that CST 3 may affect endothelial function and angiogenic capacity. In the current study, we sought to determine the influence of CST 3 on endothelial function and explore its potential regulatory pathway. Methods and Results We analyzed CST 3 and vascular endothelial growth factor A ( VEGFA) levels in different developmental stages of gerbils using ELISA s and immunofluorescence (to examine the relationship between CST 3 and VEGFA . We used a real-time cell analyzer, cytotoxicity assays, and the chorioallantoic membrane assay to investigate the function of CST 3 in endothelial cells and the chorioallantoic membrane. Additionally, we used Western blotting to explore the downstream targets of CST 3. The expression levels of both CST 3 and VEGFA were at their highest on day 10 of the embryonic stage. CST 3 inhibited endothelial cell proliferation, migration, tube formation, and permeability, as well as vascular development in the chorioallantoic membrane. Blocking of VEGFA dose-dependently increased CST 3 expression in arterial and venous endothelial cells. Furthermore, overexpression and knockdown of CST 3 significantly affected the protein levels of p53 and CAPN10 (calpain 10), suggesting that CST 3 might play a role in vascular development through these proteins. Conclusions CST 3 may be associated with vascular development and angiogenesis, and this effect could be promoted by blocking VEGFA .

Published

2018

5. Expression and significance of Cystatin-C in clear cell renal cell carcinoma.

Author

Guo K, Chen Q, He X, Yao K, Li Z, Liu Z, Chen J, Liu Z, Guo C, Lu J, Wu C, Li W, Wang Q, Chen P, Lu W, Wang Y, Han H, Cao Y, and Guo S

Subjects

Biomarkers, Tumor blood, Carcinoma, Renal Cell blood, Carcinoma, Renal Cell pathology, Cell Line, Tumor, Cell Movement, Cell Proliferation, Cystatin C blood, Cystatin C genetics, Disease-Free Survival, Female, Gene Editing, Humans, Immunohistochemistry, Kaplan-Meier Estimate, Kidney Neoplasms blood, Kidney Neoplasms pathology, Male, Middle Aged, Neoplasm Invasiveness, Sensitivity and Specificity, Biomarkers, Tumor biosynthesis, Carcinoma, Renal Cell diagnosis, Cystatin C biosynthesis, Kidney Neoplasms diagnosis

Abstract

Purpose: Cystatin-C (Cys-C) has been studied as a valuable prognostic indicator in several malignancies. The goal of this study is to explore the expression and prognostic significance of Cys-C in clear cell renal cell carcinoma (CCRCC)., Methods: Immunohistochemistry and western blot assays were performed to evaluate the level of Cys-C expression in CCRCC tissue. Expression levels of Cys-C in CCRCC tissue samples in relation to clinicopathological characteristics of the tumors were assessed. Their prognostic significance was analyzed by univariate and multivariate analyses. In addition, the expression of Cys-C in 786-O cell lines was inhibited by using CRISPR/Case9 and the effects of Cys-C knockout on 786-O cells in vitro were evaluated using MTT method, colony formation assay, cell cycle assay, and cell migration and invasive assay., Results: The expression level of Cys-C was lower in CCRCC tissues (n = 253) than in paired adjacent non-cancerous tissues (n = 164) by immunohistochemistry (P < 0.001). Among the 253 patients, the results showed that patients with low Cys-C expression level in cancer tissue has longer overall survival (OS) than that with high Cys-C level. Furthermore, knockout of Cys-C in 786-O cell line has ability to suppress cell proliferation, induce G0/G1 phase arrest, inhibited cell invasion, decreased phosphorylation of ERK1/2, STAT-3 and enhanced phosphorylated JNK expression., Conclusions: A decrease in serum Cys-C is a favorable prognostic indicator for CCRCC patients. Inhibition of Cys-C suppressed RCC 786-O cell proliferation and invasion. These results indicated that Cys-C could serve as an ideal prognostic biomarker in patients with CCRCC., (Copyright © 2018 The Authors. Published by Elsevier Masson SAS.. All rights reserved.)

Published

2018

6. Novel intracytoplasmic inclusions immunoreactive for phosphorylated-TDP43 and cystatin C in anterior horn cells in a case of sporadic amyotrophic lateral sclerosis.

Author

Shintaku M, Kaneda D, and Oyanagi K

Subjects

Amyotrophic Lateral Sclerosis metabolism, Anterior Horn Cells metabolism, Female, Humans, Inclusion Bodies metabolism, Middle Aged, Phosphorylation, Amyotrophic Lateral Sclerosis pathology, Anterior Horn Cells pathology, Cystatin C biosynthesis, DNA-Binding Proteins biosynthesis, Inclusion Bodies pathology

Abstract

Novel intracytoplasmic inclusions immunoreactive for phosphorylated transactivation response DNA-binding protein 43 (p-TDP43), cystatin C, and transferrin were found in anterior horn cells in a case of sporadic amyotrophic lateral sclerosis (ALS). The patient was a 59-year-old woman, who died of ALS after a clinical course of 8 years. She had been receiving mechanical support for respiration for 6 years and in a "totally locked-in" state for 4 years prior to death. The spinal cord showed severe degeneration involving the anterior and lateral funiculi, whereas the posterior funiculus was preserved. Neurons in the anterior horn and Clarke's column were markedly lost, and many Bunina bodies and a few skein-like inclusions were found. Some remaining anterior horn cells had round and densely eosinophilic or amphophilic intracytoplasmic inclusions. They were immunoreactive for ubiquitin, p-TDP43, cystatin C and transferrin. On confocal laser microscopy, cystatin C was found to consistently surround p-TDP43 within the inclusions. The inclusions ultrastructurally consisted of granule-associated fibrils and, in the central portion, dense aggregates of fibrils were associated with masses of electron-dense, coarsely granular or amorphous material. Although their pathogenesis remains unknown, these unique inclusions may have been formed under a specific condition whereby p-TDP43 and cystatin C interacted with each other., (© 2017 Japanese Society of Neuropathology.)

Published

2017

7. Expression, purification, and characterization of human cystatin C monomers and oligomers.

Author

Perlenfein TJ and Murphy RM

Subjects

Humans, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Cystatin C biosynthesis, Cystatin C chemistry, Cystatin C genetics, Cystatin C isolation & purification, Gene Expression, Protein Folding, Protein Multimerization

Abstract

Human cystatin C (cysC) is a soluble basic protein belonging to the cysteine protease inhibitor family. CysC is a potent inhibitor of cathepsins--proteolytic enzymes that degrade intracellular and endocytosed proteins, remodel extracellular matrix, and trigger apoptosis. Inhibition is via tight reversible binding involving the N-terminus as well as two β-hairpin loops of cysC. As a significant component of cerebrospinal fluid, cysC has numerous other functions, including support of neural stem cell growth and differentiation. Several studies suggest that cysC may bind to the Alzheimer-related protein beta-amyloid (Aβ), and inhibit its aggregation and toxicity. Because of an increasing recognition of its important biological roles, there is considerable interest in methods to produce full-length recombinant human cysC. Several researchers have reported success, but with processes that require multiple purification steps. Here we report successful production of human cysC using an intein-based expression system and a simple one-column purification scheme. The recombinant protein so obtained was natively folded and active as an enzyme inhibitor. Unexpectedly, even mild concentration by ultrafiltration caused significant oligomerization. The oligomers are noncovalent and retain the native secondary structure and inhibitory activity of the monomer. The oligomers, but not the monomers, were highly effective at inhibiting aggregation of Aβ. These results demonstrate the critical importance of careful physicochemical characterization of recombinant cysC protein prior to evaluation of its biological functions., (Copyright © 2015 Elsevier Inc. All rights reserved.)

Published

2016

8. Efficient expression, purification and characterization of native human cystatin C in Escherichia coli periplasm.

Author

Zhou Y, Zhou Y, Li J, Chen J, Yao Y, Yu L, Peng D, Wang M, Su D, He Y, and Gou L

Subjects

Cystatin C genetics, Escherichia coli genetics, Humans, Periplasm genetics, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Cystatin C biosynthesis, Cystatin C chemistry, Cystatin C isolation & purification, Escherichia coli metabolism, Gene Expression, Periplasm metabolism

Abstract

Human cystatin C (HCC), encoded by cystatin 3 gene, is a 13.3kDa endogenous cysteine proteinase inhibitor and an important biomarker of renal function. However, expressing recombinant cystatin C is difficult because of low yield and inclusion bodies in Escherichia coli (E. coli). In this study, we cloned HCC gene into pET-22b vector containing PelB leader signal sequence, which could direct the protein to the bacterial periplasm. Large amounts of soluble HCC could be efficiently expressed in the bacterial periplasm at 16°C with 0.1mM IPTG induction. The recombinant HCC was isolated in high purity by cation exchange chromatography and gel filtration chromatography. Furthermore, the HCC was characterized by circular dichroism (CD) and dynamic light scattering (DLS), and displayed biological activity against papain. Here, we provide a method to produce large amounts of soluble mature HCC in E. coli., (Copyright © 2015 Elsevier Inc. All rights reserved.)

Published

2015

9. Analysis of protein expression changes of the Vero E6 cells infected with classic PEDV strain CV777 by using quantitative proteomic technique.

Author

Sun D, Shi H, Guo D, Chen J, Shi D, Zhu Q, Zhang X, and Feng L

Subjects

Animals, CD18 Antigens biosynthesis, Chlorocebus aethiops, Coronavirus Infections virology, Cystatin C biosynthesis, Gene Expression, Gene Expression Profiling, Integrin beta3 biosynthesis, Porcine epidemic diarrhea virus metabolism, Proteomics methods, Swine virology, Swine Diseases virology, Vero Cells, Viral Proteins biosynthesis, Coronavirus Infections pathology, Coronavirus Infections veterinary, Viral Proteins metabolism

Abstract

Recent outbreaks of porcine epidemic diarrhea virus (PEDV) have caused widespread concern. The identification of proteins associated with PEDV infection might provide insight into PEDV pathogenesis and facilitate the development of novel antiviral strategies. We analyzed the differential protein profile of PEDV-infected Vero E6 cells using mass spectrometry and an isobaric tag for relative and absolute quantification. A total of 126 proteins were identified that were differentially expressed between the PEDV-infected and mock-infected groups (P<0.05, quantitative ratio ≥1.2), among which the expression of 58 proteins was up-regulated and that of 68 proteins was down-regulated in the PEDV-infected Vero E6 cells, involving in integrin β2/β3, cystatin-C. The Gene Ontology analysis indicated that the molecular function of the differentially expressed proteins (DEPs) was primarily related to binding and catalytic activity, and that the biological functions in which the DEPs are involved included metabolism, organismal systems, cellular processes, genetic information processing, environmental information processing, and diseases. Among the disease-related functions, certain anti-viral pathways and proteins, such as the RIG-I-like receptor, Rap1, autophagy, mitogen-activated protein kinase, PI3K-Akt and Jak-STAT signaling pathways, and integrin β2/β3 and cystatin-C proteins, represented potential factors in PEDV infection. Our findings provide valuable insight into PEDV-Vero E6 cell interactions., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published

2015

10. Overexpression of cystatin C in synovium does not reduce synovitis or cartilage degradation in established osteoarthritis.

Author

Kyostio-Moore S, Piraino S, Berthelette P, Moran N, Serriello J, Bendele A, Sookdeo C, Nambiar B, Ewing P, Armentano D, and Matthews GL

Subjects

Animals, Cartilage, Articular pathology, Gene Expression Regulation, Humans, Male, Osteoarthritis pathology, Rabbits, Synovial Membrane pathology, Synovitis pathology, Cartilage, Articular metabolism, Cystatin C biosynthesis, Osteoarthritis metabolism, Synovial Membrane metabolism, Synovitis metabolism

Abstract

Introduction: Cathepsin K (catK) expression is increased in cartilage, bone and synovium during osteoarthritis (OA). To study the role of catK expression and elevated cathepsin activity in the synovium on cartilage destruction in established OA, we overexpressed cystatin C (cysC), a natural cysteine protease inhibitor, in the synovium of rabbit OA joints., Methods: The ability of cysC to inhibit activity of cathepsins in rabbit OA synovium lysates was tested in vitro using protease activity assay. In vivo, the tissue localization of recombinant adeno-associated virus (rAAV) with LacZ gene after intra-articular injection was determined by β-galactosidase staining of rabbit joints 4 weeks later. To inhibit cathepsin activity in the synovium, a rAAV2-encoding cysC was delivered intra-articularly into rabbit joints 4 weeks after OA was induced by anterior cruciate ligament transection (ACLT). Seven weeks postinjection, endogenous catK and cysC levels as well as the vector-derived cysC expression in the synovium of normal and OA joints were examined by RNA quantification. Synovial cathepsin activity and catK, catB and catL protein levels were determined by activity and Western blot analyses, respectively. Synovitis and cartilage degradation were evaluated by histopathological scoring., Results: In vitro, the ability of cysC to efficiently inhibit activity of purified catK and OA-induced cathepsins in rabbit synovial lysates was demonstrated. In vivo, the intra-articular delivery of rAAV2/LacZ showed transduction of mostly synovium. Induction of OA in rabbit joints resulted in fourfold increase in catK mRNA compared to sham controls while no change was detected in endogenous cysC mRNA levels in the synovium. Protein levels for catK, catB and catL were also increased in the synovium with a concomitant fourfold increase in cathepsin activity. Joints treated with rAAV2/cysC showed both detection of vector genomes and vector-derived cysC transcripts in the synovium. Production of functional cysC by the vector was demonstrated by complete block of cathepsin activity in the synovium. However, this did not decrease synovitis, bone sclerosis or progression of cartilage degradation., Conclusions: Increased production of natural cathepsin inhibitor, cysC, in OA synovium does not alleviate synovitis or cartilage pathology during a preexisting OA.

Published

2015

11. Expression and purification of soluble human cystatin C in Escherichia coli with maltose-binding protein as a soluble partner.

Author

Zhang Q, Zhao X, Xu X, Tang B, Zha Z, Zhang M, Yao D, Chen X, Wu X, Cao L, and Guo H

Subjects

Cathepsin B metabolism, Chromatography, Affinity, Cystatin C genetics, Cystatin C isolation & purification, Escherichia coli, Glutathione Transferase genetics, Humans, Papain metabolism, Prokaryotic Initiation Factor-2 genetics, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins isolation & purification, Solubility, Cystatin C biosynthesis, Maltose-Binding Proteins genetics, Recombinant Fusion Proteins biosynthesis

Abstract

Human cystatin C (CYSC) is a 13-kDa endogenous cysteine proteinase inhibitor and was investigated as a replacement for creatinine as a marker of renal function. However, expressing recombinant CYSC is difficult in Escherichia coli because of resulting low yield and insufficient purity and insolubility. Here, we cloned and fused CYSC to the C-terminus of three soluble partners - maltose-binding protein (MBP), glutathione S-transferase (GST) and translation initiation factor 2 domain I (IF2) - to screen for their ability to improve the solubility of recombinant CYSC when expressed in E. coli. MBP was best at enhancing the soluble expression of CYSC, with soluble fractions accounting for 92.8±3.11% of all proteins. For scaled production, we purified the de-tagged CYSC by using a 3C protease-cleaved MBP-T3-CYSC fused protein with immobilized metal affinity chromatography and cation-affinity purification. The molecular weights of the de-tagged CYSC and human natural CYSC were similar, and the former could react specifically with CYSC polyclonal antibody. Moreover, the de-tagged CYSC displayed full biological activity against papain and cathepsin B, which was very similar to that of the human natural CYSC protein standard. We provide a method to produce large amounts of soluble recombinant human CYSC in E. coli., (Copyright © 2014 Elsevier Inc. All rights reserved.)

Published

2014

12. Genetic regulation of gene expression in the lung identifies CST3 and CD22 as potential causal genes for airflow obstruction.

Author

Lamontagne M, Timens W, Hao K, Bossé Y, Laviolette M, Steiling K, Campbell JD, Couture C, Conti M, Sherwood K, Hogg JC, Brandsma CA, van den Berge M, Sandford A, Lam S, Lenburg ME, Spira A, Paré PD, Nickle D, Sin DD, and Postma DS

Subjects

Cystatin C biosynthesis, Female, Genome-Wide Association Study, Genotype, Humans, Male, Middle Aged, Phenotype, Polymorphism, Single Nucleotide, Pulmonary Disease, Chronic Obstructive metabolism, Pulmonary Disease, Chronic Obstructive physiopathology, Reproducibility of Results, Sialic Acid Binding Ig-like Lectin 2 biosynthesis, Cystatin C genetics, Forced Expiratory Volume physiology, Gene Expression Regulation, Genetic Predisposition to Disease, Pulmonary Disease, Chronic Obstructive genetics, RNA, Messenger genetics, Sialic Acid Binding Ig-like Lectin 2 genetics

Abstract

Background: COPD is a complex chronic disease with poorly understood pathogenesis. Integrative genomic approaches have the potential to elucidate the biological networks underlying COPD and lung function. We recently combined genome-wide genotyping and gene expression in 1111 human lung specimens to map expression quantitative trait loci (eQTL)., Objective: To determine causal associations between COPD and lung function-associated single nucleotide polymorphisms (SNPs) and lung tissue gene expression changes in our lung eQTL dataset., Methods: We evaluated causality between SNPs and gene expression for three COPD phenotypes: FEV(1)% predicted, FEV(1)/FVC and COPD as a categorical variable. Different models were assessed in the three cohorts independently and in a meta-analysis. SNPs associated with a COPD phenotype and gene expression were subjected to causal pathway modelling and manual curation. In silico analyses evaluated functional enrichment of biological pathways among newly identified causal genes. Biologically relevant causal genes were validated in two separate gene expression datasets of lung tissues and bronchial airway brushings., Results: High reliability causal relations were found in SNP-mRNA-phenotype triplets for FEV(1)% predicted (n=169) and FEV(1)/FVC (n=80). Several genes of potential biological relevance for COPD were revealed. eQTL-SNPs upregulating cystatin C (CST3) and CD22 were associated with worse lung function. Signalling pathways enriched with causal genes included xenobiotic metabolism, apoptosis, protease-antiprotease and oxidant-antioxidant balance., Conclusions: By using integrative genomics and analysing the relationships of COPD phenotypes with SNPs and gene expression in lung tissue, we identified CST3 and CD22 as potential causal genes for airflow obstruction. This study also augmented the understanding of previously described COPD pathways., (Published by the BMJ Publishing Group Limited. For permission to use (where not already granted under a licence) please go to http://group.bmj.com/group/rights-licensing/permissions.)

Published

2014

13. Increased expression of cystatin C and transforming growth factor β-1 in calcific aortic valves.

Author

Yetkin E, Tchaikovski V, Erdil N, Alan S, and Waltenberger J

Subjects

Animals, Aortic Valve Stenosis pathology, Blotting, Western, Calcinosis pathology, Humans, Immunohistochemistry, Aortic Valve metabolism, Aortic Valve pathology, Aortic Valve Stenosis metabolism, Calcinosis metabolism, Cystatin C biosynthesis, Transforming Growth Factor beta1 biosynthesis

Published

2014

14. Effect of codon optimization on expression levels of human cystatin C in Pichia pastoris.

Author

Li YM, Li DJ, Xu XJ, Cui M, Zhen HH, and Wang Q

Subjects

Amino Acid Sequence, Base Composition, Base Sequence, Cystatin C biosynthesis, Cystatin C chemistry, Gene Expression, Humans, Molecular Sequence Data, Pichia metabolism, Protein Engineering, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins genetics, Cloning, Molecular methods, Codon, Cystatin C genetics, Pichia genetics

Abstract

Human cystatin C (CysC) is a cysteine proteinase inhibitor with many potential applications. To facilitate further studies of the functions and applications of CysC, we improved the heterologous expression of CysC using a basic codon optimization method. In this study, we cloned the high-GC content wild-type sequence of the CysC gene and also designed a slightly AT-biased sequence, with codons optimized for expression in the Pichia pastoris GS115 strain. Our results showed that the optimized coding sequence of human CysC increased the expression and secretion of the CysC protein by approximately 3- to 5-fold (90-96 mg CysC/L) in yeast, compared with the expression levels of the native CysC gene (17.9-18.4 mg CysC/L). We designed, constructed, and applied an optimized version of the CysC gene for the Pichia expression system. Our results demonstrate that the optimized coding sequence provides a higher yield of secreted CysC than that produced using the wild-type gene. Our data also serve as a practical example demonstrating a rational design strategy for the heterologous expression of secreted proteins.

Published

2014

15. Developmental regulation of synthesis and dimerization of the amyloidogenic protease inhibitor cystatin C in the hematopoietic system.

Author

Xu Y, Lindemann P, Vega-Ramos J, Zhang JG, and Villadangos JA

Subjects

Animals, Cystatin C genetics, Dendritic Cells cytology, Dendritic Cells metabolism, Endoplasmic Reticulum genetics, Endoplasmic Reticulum metabolism, Hematopoiesis physiology, Hematopoietic Stem Cells cytology, Inflammation genetics, Inflammation metabolism, Macrophages cytology, Macrophages metabolism, Mice, Mice, Mutant Strains, Mitochondria genetics, Mitochondria metabolism, Reactive Oxygen Species metabolism, Cystatin C biosynthesis, Hematopoietic Stem Cells metabolism, Protein Biosynthesis physiology, Protein Multimerization physiology

Abstract

The cysteine protease inhibitor cystatin C is thought to be secreted by most cells and eliminated in the kidneys, so its concentration in plasma is diagnostic of kidney function. Low extracellular cystatin C is linked to pathologic protease activity in cancer, arthritis, atherosclerosis, aortic aneurism, and emphysema. Cystatin C forms non-inhibitory dimers and aggregates by a mechanism known as domain swapping, a property that reportedly protects against Alzheimer disease but can also cause amyloid angiopathy. Despite these clinical associations, little is known about the regulation of cystatin C production, dimerization, and secretion. We show that hematopoietic cells are major contributors to extracellular cystatin C levels in healthy mice. Among these cells, macrophages and dendritic cells (DC) are the predominant producers of cystatin C. Both cell types synthesize monomeric and dimeric cystatin C in vivo, but only secrete monomer. Dimerization occurs co-translationally in the endoplasmic reticulum and is regulated by the levels of reactive oxygen species (ROS) derived from mitochondria. Drugs or stimuli that reduce the intracellular concentration of ROS inhibit cystatin C dimerization. The extracellular concentration of inhibitory cystatin C is thus partly dependent on the abundance of macrophages and DC, and the ROS levels. These results have implications for the diagnostic use of serum cystatin C as a marker of kidney function during inflammatory processes that induce changes in DC or macrophage abundance. They also suggest an important role for macrophages, DC, and ROS in diseases associated with the protease inhibitory activity or amyloidogenic properties of cystatin C.

Published

2014

16. Cystatin C has a dual role in post-traumatic brain injury recovery.

Author

Martinez-Vargas M, Soto-Nuñez M, Tabla-Ramon E, Solis B, Gonzalez-Rivera R, Perez-Arredondo A, Estrada-Rojo F, Castell A, Molina-Guarneros J, and Navarro L

Subjects

Animals, Apoptosis, Brain Stem metabolism, Cathepsin B metabolism, Cerebellum metabolism, Cerebral Cortex metabolism, Choroid Plexus metabolism, Cystatin C biosynthesis, Hemorrhage chemically induced, Hippocampus metabolism, Male, Neurons pathology, Rats, Rats, Wistar, Brain Injuries mortality, Brain Injuries pathology, Cathepsin B biosynthesis, Cystatin C pharmacology

Abstract

Cathepsin B is one of the major lysosomal cysteine proteases involved in neuronal protein catabolism. This cathepsin is released after traumatic injury and increases neuronal death; however, release of cystatin C, a cathepsin inhibitor, appears to be a self-protective brain response. Here we describe the effect of cystatin C intracerebroventricular administration in rats prior to inducing a traumatic brain injury. We observed that cystatin C injection caused a dual response in post-traumatic brain injury recovery: higher doses (350 fmoles) increased bleeding and mortality, whereas lower doses (3.5 to 35 fmoles) decreased bleeding, neuronal damage and mortality. We also analyzed the expression of cathepsin B and cystatin C in the brains of control rats and of rats after a traumatic brain injury. Cathepsin B was detected in the brain stem, cerebellum, hippocampus and cerebral cortex of control rats. Cystatin C was localized to the choroid plexus, brain stem and cerebellum of control rats. Twenty-four hours after traumatic brain injury, we observed changes in both the expression and localization of both proteins in the cerebral cortex, hippocampus and brain stem. An early increase and intralysosomal expression of cystatin C after brain injury was associated with reduced neuronal damage.

Published

2014

17. Serum cystatin C concentrations are increased in human obesity in relation to over-production by the adipose tissue.

Author

Guerre-Millo M

Subjects

Body Mass Index, Female, Glomerular Filtration Rate, Humans, Male, Obesity blood, Adipose Tissue metabolism, Cystatin C biosynthesis, Cystatin C blood, Obesity metabolism

Published

2012

18. [Fundamental and clinical aspects of cystatin C].

Author

Itoh Y, Kawabata I, Akasaka K, and Kino S

Subjects

Biomarkers blood, Glomerular Filtration Rate, Humans, Immunoassay, Reference Values, Cystatin C biosynthesis, Cystatin C chemistry, Kidney Function Tests

Abstract

Recent progress of fundamental and clinical studies on cystatin C was reviewed. Most of key studies are indebted to prof. Grubb A and his groups. International contributions from Japanese research work are included here. The protein is a basic low molecular weight protein of 13,300 with 120 amino acid residues and pI 9.3, functioning as a cysteine protease inhibitor. With an introduction of ERM-DA471, international reference material for serum cystatin C, global standardization for immunoassay systems has been much facilitated. No serious problems are present in the pre-analytical stage. Serum reference intervals are properly set in all Asian populations including Japanese with age and gender-related differences. The protein is a powerful serum intrinsic marker for glomerular filtration rate. Estimated glomerular filtration rate (eGFRcysC) in coupled with eGFRCr will definitely be a clinical routine for early detection and prevention of altered kidney function and cardiovascular events in general population. Genetic tests clinically indicated include hereditary cystatin C amyloid angiopathy (L68Q) and adult macular degeneration (A25T) although their frequency is extremely low.

Published

2012

19. Triiodothyronine stimulates cystatin C production in bone cells.

Author

Schmid C, Ghirlanda-Keller C, Zwimpfer C, and Zoidis E

Subjects

Alkaline Phosphatase biosynthesis, Animals, Cells, Cultured, Deoxyglucose analogs & derivatives, Deoxyglucose metabolism, Dexamethasone pharmacology, Glucose Transporter Type 3 biosynthesis, Osteoblasts metabolism, RNA, Messenger biosynthesis, Rats, Cystatin C biosynthesis, Osteoblasts drug effects, Triiodothyronine pharmacology

Abstract

Thyroid hormones increase cystatin C levels in vivo. To study whether 3,3',5-triiodo-l-thyronine (T(3)) stimulates the production of cystatin C in vitro, we used a T(3)-responsive osteoblastic cell line (PyMS) which can be kept in serum-free culture. We compared the effects of T(3) on cystatin C mRNA expression (by Northern) and on protein release (by Western and ELISA) with those of dexamethasone (dex). Triiodothyronine increased cystatin C mRNA expression and cystatin C accumulation in culture media in a dose- and time-dependent manner, 1.5-fold at 1 nmol/l after 4d; dex (100 nmol/l) was more potent and increased cystatin C accumulation 3-fold after 4d. Triiodothyronine but not dex stimulated glucose uptake. Our in vitro findings explain in vivo observations. Triiodothyronine-induced increase in the production of cystatin C may be related to an increased cell metabolism and proteolysis control demand., (Copyright © 2012 Elsevier Inc. All rights reserved.)

Published

2012

20. Codon preference optimization increases prokaryotic cystatin C expression.

Author

Wang Q, Mei C, Zhen H, and Zhu J

Subjects

Humans, Recombinant Proteins isolation & purification, Codon genetics, Cystatin C biosynthesis, Cystatin C genetics, Escherichia coli physiology, Genetic Enhancement methods, Protein Engineering methods, Recombinant Proteins metabolism

Abstract

Gene expression is closely related to optimal vector-host system pairing in many prokaryotes. Redesign of the human cystatin C (cysC) gene using the preferred codons of the prokaryotic system may significantly increase cysC expression in Escherichia coli (E. coli). Specifically, cysC expression may be increased by removing unstable sequences and optimizing GC content. According to E. coli expression system codon preferences, the gene sequence was optimized while the amino acid sequence was maintained. The codon-optimized cysC (co-cysC) and wild-type cysC (wt-cysC) were expressed by cloning the genes into a pET-30a plasmid, thus transforming the recombinant plasmid into E. coli BL21. Before and after the optimization process, the prokaryotic expression vector and host bacteria were examined for protein expression and biological activation of CysC. The recombinant proteins in the lysate of the transformed bacteria were purified using Ni(2+)-NTA resin. Recombinant protein expression increased from 10% to 46% based on total protein expression after codon optimization. Recombinant CysC purity was above 95%. The significant increase in cysC expression in E. coli expression produced by codon optimization techniques may be applicable to commercial production systems.

Published

2012

21. Cathepsins and their endogenous inhibitors cystatins: expression and modulation in multiple sclerosis.

Author

Haves-Zburof D, Paperna T, Gour-Lavie A, Mandel I, Glass-Marmor L, and Miller A

Subjects

Adolescent, Adult, Biomarkers, Cathepsin B antagonists & inhibitors, Cathepsin B biosynthesis, Cathepsins antagonists & inhibitors, Cathepsins biosynthesis, Cystatin B biosynthesis, Cystatin B blood, Cystatin C biosynthesis, Cystatin C blood, Disease Progression, Female, Humans, Interferon-beta pharmacology, Leukocytes cytology, Male, Methylprednisolone pharmacology, Middle Aged, Multiple Sclerosis drug therapy, Multiple Sclerosis pathology, RNA, Messenger biosynthesis, Cathepsin B metabolism, Cathepsins metabolism, Cystatin B metabolism, Cystatin C metabolism, Multiple Sclerosis metabolism

Abstract

Cathepsins are involved in a variety of physiological processes including antigen processing and presentation and extracellular matrix degradation. In the present study, we evaluated whether expression levels of cathepsins S and B and their inhibitors cystatins B and C are affected by multiple sclerosis (MS) disease state (relapse and remission) and therapies (interferon-β [IFN-β] and the glucocorticoid [GC] methylprednisolone), and whether they are associated with the IFN-β response phenotype. Real-time PCR was employed to compare RNA expression levels in peripheral blood leucocytes (PBLs) and ELISA to determine serum protein levels of MS patients and matched healthy individuals. Cathepsin S RNA was higher in MS patients in the relapse state compared to controls (by 74%, P = 3 × 10(-5), n = 30 versus n = 18) with a similar increase observed in serum (66%, P = 0.002, n = 18 versus n = 20). GC treatment reduced cathepsin S levels in PBL RNA (by 44%, P = 6 × 10(-6), n = 27) and serum proteins (by 27%, P = 1 × 10(-5), n = 26), reduced the serum protein levels of pro-cathepsin B (by 8%, P = 0.0007, n = 23), and in parallel increased the serum levels of their inhibitor cystatin C (by 82%, P = 8 × 10(-6), n = 26). IFN-β therapy significantly elevated the RNA levels (n = 16) of cathepsin B (by 16%, P = 0.03), cystatin B (44%, P = 0.004) and cystatin C (48%, P = 0.011). In the serum, only cathepsin S levels were reduced by IFN-β (16%, P = 0.006, n = 25). Interestingly, pre-treatment serum cathepsin S/cystatin C ratio was higher in 'good responders' to IFN-β therapy compared to patients without a good response (by 94%, P = 0.003). These results suggest that cathepsin S and cystatin C may contribute to disease activity in MS, specifically in a subgroup of patients that are responsive to IFN-β therapy, and that these proteins should be further evaluated as biomarkers in MS., (© 2011 The Authors Journal of Cellular and Molecular Medicine © 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd.)

Published

2011

22. IL-10 controls cystatin C synthesis and blood concentration in response to inflammation through regulation of IFN regulatory factor 8 expression.

Author

Xu Y, Schnorrer P, Proietto A, Kowalski G, Febbraio MA, Acha-Orbea H, Dickins RA, and Villadangos JA

Subjects

Animals, Bone Marrow Transplantation immunology, Bone Marrow Transplantation pathology, Cell Line, Tumor, Cells, Cultured, Coculture Techniques, Cystatin C deficiency, Dendritic Cells classification, Dendritic Cells immunology, Dendritic Cells pathology, Down-Regulation genetics, Inflammation Mediators antagonists & inhibitors, Interferon Regulatory Factors deficiency, Interferon Regulatory Factors physiology, Interleukin-10 metabolism, Melanoma, Experimental, Mice, Mice, Inbred C57BL, Mice, Knockout, Mice, Transgenic, Cystatin C biosynthesis, Cystatin C blood, Down-Regulation immunology, Inflammation Mediators physiology, Interferon Regulatory Factors biosynthesis, Interleukin-10 physiology

Abstract

Cystatin C (CstC) is a cysteine protease inhibitor of major clinical importance. Low concentration of serum CstC is linked to atherosclerosis. CstC can prevent formation of amyloid β associated with Alzheimer's disease and can itself form toxic aggregates. CstC regulates NO secretion by macrophages and is a TGF-β antagonist. Finally, the serum concentration of CstC is an indicator of kidney function. Yet, little is known about the regulation of CstC expression in vivo. In this study, we demonstrate that the transcription factor IFN regulatory factor 8 (IRF-8) is critical for CstC expression in primary dendritic cells. Only those cells with IRF-8 bound to the CstC gene promoter expressed high levels of the inhibitor. Secretion of IL-10 in response to inflammatory stimuli downregulated IRF-8 expression and consequently CstC synthesis in vivo. Furthermore, the serum concentration of CstC decreased in an IL-10-dependent manner in mice treated with the TLR9 agonist CpG. CstC synthesis is therefore more tightly regulated than hitherto recognized. The mechanisms involved in this regulation might be targeted to alter CstC production, with potential therapeutic value. Our results also indicate that caution should be exerted when using the concentration of serum CstC as an indicator of kidney function in conditions in which inflammation may alter CstC production.

Published

2011

23. Amino-terminal pro-brain natriuretic peptide as a prognostic marker in patients with rheumatoid arthritis.

Author

Targońska-Stępniak B and Majdan M

Subjects

Adolescent, Adult, Blood Sedimentation, C-Reactive Protein biosynthesis, Cardiovascular Diseases complications, Cystatin C biosynthesis, Female, Humans, Male, Middle Aged, Prognosis, Tunica Intima pathology, Tunica Media pathology, Ultrasonography methods, Arthritis, Rheumatoid blood, Arthritis, Rheumatoid diagnosis, Natriuretic Peptide, Brain biosynthesis, Peptide Fragments biosynthesis

Abstract

Rheumatoid arthritis (RA) is associated with increased cardiovascular (CV) morbidity and mortality, of which amino-terminal pro-brain natriuretic peptide (NT-proBNP) is a predictor. The objective of the study was to investigate associations between NT-proBNP and age, gender, markers of inflammation, disease activity, and kidney function in RA patients, without co-morbidities potentially influencing NT-proBNP concentration. The study group consisted of 90 patients with RA, without clinically relevant coronary heart disease, hypertension, diabetes, advanced chronic kidney disease. The comprehensive assessment of clinical and laboratory parameters of inflammation, disease activity, and kidney function was performed. Plasma samples were frozen for NT-proBNP analysis. Carotid intima media thickness (cIMT) was determined by high-resolution B-mode ultrasonography. The mean NT-proBNP concentrations were significantly higher in a group of RA patients with high disease activity (DAS28 > 5.1) and in a group of patients with subclinical atherosclerosis diagnosed by cIMT ≥ 0.6 mm. In all RA patients, NT-proBNP correlated positively with the age, C-reactive protein, erythrocyte sedimentation rate, cIMT, tricipital skin fold and negatively with hand-grip strength, hemoglobin, red blood cell count, albumin. In the group of women with RA, we found significant positive correlation between NT-proBNP and cystatin-C. Also, patients with NT-proBNP level ≥ 100 pg/ml had significantly higher cystatin-C than those with lower NT-proBNP. NT-proBNP level, in RA patients without co-morbidities potentially influencing this level, is correlated with age, disease activity markers of inflammation, and subclinical renal impairment. It means that risk of CV disorders is higher in older patients with more active RA.

Published

2011

24. Mild renal dysfunction as a non-traditional cardiovascular risk factor?-Association of cystatin C-based glomerular filtration rate with flow-mediated vasodilation.

Author

Reffelmann T, Krebs A, Ittermann T, Empen K, Hummel A, Dörr M, Völzke H, and Felix SB

Subjects

Biomarkers, Brachial Artery pathology, Female, Humans, Kidney pathology, Male, Middle Aged, Risk Factors, Cardiovascular Diseases complications, Cardiovascular Diseases pathology, Cystatin C biosynthesis, Glomerular Filtration Rate, Kidney Diseases complications, Kidney Diseases pathology, Vasodilation

Abstract

Objective: Chronic kidney disease, at least in its advanced stages, can be regarded as a non-traditional cardiovascular risk factor. The purpose of this study was to evaluate whether early stages of renal dysfunction are associated with flow-mediated vasodilatation, as an early marker of the atherosclerotic disease process., Methods: In 1515 subjects (753 females) from the population-based Study of Health in Pomerania, the relationship between flow-mediated vasodilatation of the brachial artery (cuff occlusion of the forearm for 5 min) and glomerular filtration rate, estimated on the basis of serum cystatin C levels, was analyzed under consideration of various cardiovascular risk factors., Results: Flow-mediated vasodilatation was 5.75 + or - 0.16% in women and 4.29+/-0.12% in men (mean + or - SEM). Glomerular filtration rate amounted to 94.2 + or - 0.7 ml/min/1.73 m(2), with 8.1% subjects with glomerular filtration rate < or = 60 ml/min/1.73 m(2). Flow-mediated vasodilatation significantly correlated with glomerular filtration rate in the entire population (r=0.237, p<0.001), in women (r=0.224, p<0.001) and in men (r=0.168, p<0.001). Adjusting for age and multiple cardiovascular risk factors and also for high-sensitive C-reactive protein levels revealed a significant association of flow-mediated vasodilatation and glomerular filtration rate in women (p=0.01), but not in men, with similar results when the analyses were restricted to individuals with glomerular filtration rate >60 ml/min/1.73 m(2)., Conclusion: Mild reduction in renal function is associated with alterations in endothelial function in females. Hence, very mild alterations in kidney function may also be regarded as a cardiovascular risk factor at least in women., (Copyright 2010 Elsevier Ireland Ltd. All rights reserved.)

Published

2010

25. Macrophage responses to interferon-gamma are dependent on cystatin C levels.

Author

Frendéus KH, Wallin H, Janciauskiene S, and Abrahamson M

Subjects

Animals, Cystatin C biosynthesis, Cystatin C deficiency, Down-Regulation drug effects, Humans, Interleukin-10 genetics, Interleukin-10 metabolism, Macrophage Activation drug effects, Macrophages cytology, Macrophages drug effects, Macrophages enzymology, Mice, Nitric Oxide Synthase Type II genetics, Nitric Oxide Synthase Type II metabolism, RNA, Messenger genetics, RNA, Messenger metabolism, Transcription Factor RelA metabolism, Tumor Necrosis Factor-alpha genetics, Tumor Necrosis Factor-alpha metabolism, Cystatin C metabolism, Interferon-gamma pharmacology, Macrophages metabolism

Abstract

The aim of the present investigation was to elucidate possible effects of cystatin C on inflammatory responses mediated by macrophages. Previously it has been shown that in vitro treatment of murine peritoneal macrophages with interferon-gamma (IFN-gamma) causes a down-regulation of cystatin C secretion. To investigate whether such changes in cystatin C expression in turn can affect inflammatory responses mediated by macrophages, we have compared effects of IFN-gamma on macrophages isolated from wild-type (cysC(+/+)) and cystatin C knockout (cysC(-/-)) mice. It was shown that IFN-gamma-primed cysC(-/-) macrophages exhibit significantly higher interleukin-10 (IL-10) but lower tumor necrosis factor-alpha (TNF-alpha) expression, and reduced nuclear factor (NF)-kappaB p65 activation, compared to similarly primed cysC(+/+) cells. Exogenously added cystatin C enhanced IFN-gamma-induced activation of NF-kappaB p65 and increased mRNA levels for inducible NO synthase (iNOS) in cysC(-/-) macrophages as well as levels of nitric oxide and TNF-alpha in the cell culture medium, in agreement with an enhanced pro-inflammatory response. Accordingly, IFN-gamma-induced IL-10 mRNA expression in cysC(-/-) macrophages was down-regulated by exogenously added cystatin C. Taken together, our data provide evidence that changes in cystatin C levels alter macrophage responses to IFN-gamma. The latter down-regulates the production of cystatin C, which leads to a suppressed inflammatory condition with enhanced IL-10 levels and down-regulated TNF-alpha and NF-kappaB. It is concluded that cystatin C through this effect can act as an immunomodulatory molecule.

Published

2009

26. Plasminogen activator inhibitor-2, but not cystatin C, inhibits the prometastatic activity of tissue inhibitor of metalloproteinases-1 in the liver.

Author

Kopitz C, Gerg M, Gansbacher B, and Krüger A

Subjects

Animals, Cell Line, Tumor, Cysteine Endopeptidases metabolism, Fibrosarcoma pathology, Humans, Liver Neoplasms pathology, Liver Neoplasms secondary, Mice, Mice, Nude, Neoplasm Metastasis, Plasminogen Activators metabolism, Cystatin C biosynthesis, Fibrosarcoma metabolism, Gene Expression Regulation, Neoplastic, Liver Neoplasms metabolism, Plasminogen Activator Inhibitor 2 biosynthesis, Tissue Inhibitor of Metalloproteinase-1 biosynthesis

Abstract

Formation of multiple and scattered metastases in target organs, leading to disruption of organ functional integrity, is the death-determining step for most lethal cancers. In the clinic, elevated expression of tissue inhibitor of metalloproteinases-1 (TIMP-1) is often associated with increased aggressiveness of cancer. We demonstrated that elevated host expression of TIMP-1 leads to the promotion of scattered liver metastases in mice, associated with increased activity of cysteine proteases (CPs). This study aimed for reduction of TIMP-1-promoted experimental liver metastases of lacZ-tagged human fibrosarcoma cells by overexpression of cystatin C, a natural inhibitor of CPs, in the murine host. Although CP inhibition reduced TIMP-induced proteolytic activity, the TIMP-1-induced increase in total tumor cell burden in livers was not significantly reduced. However, overexpression of cystatin C in livers with elevated TIMP-1 led to the formation of large multicellular metastatic foci in 42% of the mice. This formation was associated with increased expression of plasminogen activators (PAs). Additional overexpression of plasminogen activator inhibitor-2 prevented the formation of macrometastatic foci as well as the TIMP-1-induced increase in total tumor cell burden. This demonstrates that PAs are crucial for the prometastatic activity of TIMP-1 and led to the assumption that patients with elevated TIMP-1 expression may benefit from an antiproteolytic treatment directed against PAs.

Published

2008