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Query: UMLS:C0019204 (
hepatocellular carcinoma
)
71,386
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
A basic phosphoprotein defined by a monoclonal antibody named AF5 was found to be highly abundant in human
hepatocellular carcinoma
by Western immunoblotting. Under the same conditions, the levels of this phosphoprotein were low or undetectable in normal liver extracts. The AF5 antibody was used to screen a cDNA expression library of a human
hepatoma
cell line named FOCUS. A 960-base-pair cDNA was isolated and found to be a partial cDNA encoding the human protein-tyrosine kinase substrate p36, also known as
lipocortin II
. p36 expression was highly abundant in hepatocellular carcinomas at both the transcript and protein levels. Its expression was not induced significantly during rat liver regeneration following a partial hepatectomy. These results suggest that the induction of p36 expression is associated with malignant transformation of hepatocytes. p36 was previously shown to be phosphorylated upon transformation of normal fibroblasts by retroviral oncogenes without significant modulation of expression. We report here the initial description of the association of increased p36 expression with malignant transformation.
...
PMID:Enhanced expression of the protein kinase substrate p36 in human hepatocellular carcinoma. 216 May 96
The metalloproteome is defined as the set of proteins that have metal-binding capacity by being metalloproteins or having metal-binding sites. A different metalloproteome may exist for each metal. Mass spectrometric characterization of metalloproteomes provides valuable information relating to cellular disposition of metals physiologically and in metal-associated diseases. We examined the Cu and Zn metalloproteomes in three human
hepatoma
lines: Hep G2 and Mz-Hep-1, which retain many functional characteristics of normal human hepatocytes, and SK-Hep-1, which is poorly differentiated. Additionally we studied a single specimen of normal human liver and Hep G2 cells depleted in vitro of cellular copper. We used matrix-assisted laser desorption ionization and electrospray ionization quadrupole time-of-flight mass spectrometry to analyze peptide sequences of tryptic digests obtained by either in-gel digestion of metal-binding proteins or peptides on an immobilized metal affinity chromatography column loaded with either Cu or Zn. Mainly high abundance proteins were identified. Cu-binding proteins identified included enolase, albumin, transferrin, and alcohol dehydrogenase as well as certain intracellular chaperone proteins. The Cu metalloproteome was not identical to the Zn metalloproteome. Peptide binding experiments demonstrated that Cu coordination prefers the order of residues histidine > methionine > cysteine. Although the Cu metalloproteome was similar from line to line, subtle differences were apparent. Gel profiling showed more extensive variation in expression of
annexin II
in SK-Hep-1 and Mz-Hep-1 than in Hep G2 and normal liver tissue. Glycerylphosphorylethanolamine was identified as a post-translational modification at residue Glu-301 of elongation factor 1-alpha in Hep G2. Intracellular copper depletion was associated with loss of the glycerylphosphoryl side group. These findings suggest that post-translational modification could be affected by intracellular actions of copper. Comparison of the Cu and Zn metalloproteomes in Hep G2 with a published general proteome of Hep G2 disclosed little overlap (Seow, T. K., et al. (2001) Proteomics 1, 1249-1263). Proteins in the metalloproteomes of human hepatocytes can be identified by these methods. Variations in these metalloproteomes may have important physiological relevance.
...
PMID:Identification of metal-binding proteins in human hepatoma lines by immobilized metal affinity chromatography and mass spectrometry. 1453 51
Liver cancer is one of the leading causes of cancer death worldwide. To identify novel target genes that are related to liver carcinogenesis, we examined new genes that are differentially expressed in human
hepatocellular carcinoma
(
HCC
) cell lines and tissues based on the expressed sequence tag (EST) frequency. Eleven libraries were constructed from seven
HCC
cell lines and three normal liver tissue samples obtained from Korean patients. An analysis of gene expression profiles for
HCC
was performed using the frequency of ESTs obtained from these cDNA libraries. Genes were identified (n=120) as being either up- or down-regulated in human liver cancer cells. Among these, 14 genes (FTL, K-ALPHA1, LDHA, RPL4, ENO1,
ANXA2
, RPL9, RPL10, RPL13A, GNB2L1, AMBP, GC, A1BG, and SERPINC1), in addition to previously well-known liver cancer related genes, were confirmed to be differentially expressed in seven liver cancer cell lines and 17
HCC
tissues by semi-quantitative RT-PCR. In addition, 73 genes, in which there was a significant difference (P>0.99) between HBV- and HCV-associated
HCC
cells, were selected. Of these, expression patterns of 14 (RPLP0, AKR1C, KRT8, GPX4, RPS15, ID1, RPS21, VIM, EEF1G, EIF4A1, HLA-C, FN1, CD44, and RPS10) were confirmed by semi-quantitative RT-PCR in four of HBV- and three of HCV-associated
HCC
cell lines. Among those genes, an immunohistochemical analysis for
ANXA2
showed that it is expressed at high levels in
HCC
. Using an analysis of EST frequency, the newly identified genes, especially
ANXA2
, represent potential biomarkers for
HCC
and useful targets for elucidating the molecular mechanisms associated with
HCC
involving virological etiology.
...
PMID:Gene expression profiling of human HBV- and/or HCV-associated hepatocellular carcinoma cells using expressed sequence tags. 1682 Aug 72
Tumor metastasis might be associated with the expression levels of cellular glycoproteins and the alteration of their glycan parts. In order to screen the aberrantly alpha1,6-fucosylated glycoproteins related to
hepatocellular carcinoma
(
HCC
) metastasis, a high-throughput glycomic approach which consisted of 2-DE, electronic transfer of proteins, lectin affinity blot and precipitation, and MALDI-TOF-MS/MS, was established. Lens culinaris agglutinin (LCA) affinity glycoprotein profiles of higher and lower metastatic
HCC
cell lines were compared and analyzed. Seven out of 34 identified glycoproteins were differentially displayed; they were cytokeratin 8 (CK8), annexin I,
annexin II
, heterogeneous nuclear ribonucleoprotein A/B, PDZ and LIM domain 1, RNA-binding motif protein 4, and poly(rC)-binding protein 1. On comparison with Hep3B, CK8 showed a higher affinity to Ricinus communis agglutinin 1 (RCA-I) and LCA, and annexin I presented a higher affinity to LCA and Con A by the lectin-binding assay. Furthermore, the up-regulation of CK8, annexin I, and
annexin II
were found by Western blot and immunofluorescence analysis in higher metastatic
HCC
cell lines. This implied that the alteration of CK8, annexin I, and
annexin II
both in their expression levels and their glycan parts might be related to metastatic ability, and play a critical role in the process of
HCC
metastasis.
...
PMID:Identification and analysis of altered alpha1,6-fucosylated glycoproteins associated with hepatocellular carcinoma metastasis. 1706 59
The genetic background of
hepatocellular carcinoma
(
HCC
) has yet to be completely understood. Here, we describe the application of suppression subtractive hybridization (SSH) coupled with cDNA microarray analysis for the isolation and identification of differential expression of genes in
HCC
. Twenty-six known genes were validated as up-regulated and 19 known genes as down-regulated in
HCC
. The known genes identified were found to have diverse functions. In addition to the overexpression of AFP, these genes (increased in the presence of
HCC
) are involved in many processes, such as transcription and protein biosynthesis (HNRPDL, PABPC1, POLR2K, SRP9, SNRPA, and six ribosomal protein genes including RPL8, RPL14, RPL41, RPS5, RPS17, RPS24), the metabolism of lipids and proteins (FADS1, ApoA-II, ApoM, FTL), cell proliferation (Syndecan-2, and
Annexin A2
), and signal transduction (LRRC28 and FMR1). Additionally, a glutathione-binding protein involved in the detoxification of methylglyoxal known as GLO1 and an enzyme which increases the formation of prostaglandin E(2) known as PLA2G10 were up-regulated in
HCC
. Among the underexpressed genes discovered in
HCC
, most were responsible for liver-synthesized proteins (fibrinogen, complement species, amyloid, albumin, haptoglobin, hemopexin and orosomucoid). The enzyme implicated in the biotransformation of CYP family members (LOC644587) was decreased. The genes coding enzymes ADH1C, ALDH6A1, ALDOB, Arginase and CES1 were also found. Additionally, we isolated a zinc transporter (Zip14) and a function-unknown gene named ZBTB11 (Zinc finger and BTB domain containing 11) which were underexpressed, and seven expression sequence tags deregulated in
HCC
without significant homology reported in the public database. Essentially, by using SSH combined with a cDNA microarray we have identified a number of genes associated with
HCC
, most of which have not been previously reported. Further characterization of these differentially expressed genes will provide information useful in understanding the genes responsible for the development of
HCC
.
...
PMID:Identification of differential expression of genes in hepatocellular carcinoma by suppression subtractive hybridization combined cDNA microarray. 1778 58
The aim of this study was to identify molecular markers associated with oncogenic differentiation in
hepatocellular carcinoma
(
HCC
). Using an unsupervised clustering method with a cDNA microarray,
HCC
(T) gene expression profiles and corresponding non-tumor tissues (NT) from 40 patients were analyzed. Of total 217 genes, 72 were expressed preferentially in
HCC
tissues. Among 186 differentially regulated genes, there were molecular chaperone and tumor suppressor gene clusters in the Edmondson grades I and II (GI/II) subclass compared with the liver cirrhosis (LC) subclass. The Edmondson grades III and IV (GIII/IV) subclass with a poor survival (P=0.0133) contained 122 differentially regulated genes with a cluster containing various metastasis- and invasion-related genes compared with the GI/II subclass. Immunohistochemical analysis revealed that
ANXA2
, one of the 72 genes preferentially expressed in
HCC
, was over-expressed in the sinusoidal endothelium and in malignant hepatocytes in
HCC
. The genes identified in the
HCC
subclasses will be useful molecular markers for the genesis and progression of
HCC
. In addition,
ANXA2
might be a novel marker for tumor angiogenesis in
HCC
.
...
PMID:Identification of molecular markers for the oncogenic differentiation of hepatocellular carcinoma. 1805 40
DNA microarray analysis of human cancer has resulted in considerable accumulation of global gene profiles. However, extraction and understanding the underlying biology of cancer progression remains a significant challenge. This study applied a novel integrative computational and analytical approach to this challenge in human
hepatocellular carcinoma
(
HCC
) with the aim of identifying potential molecular markers or novel therapeutic targets. We analysed 100
HCC
tissue samples by human 30K DNA microarray. The gene expression data were uploaded into the network analysis tool, and the biological networks were displayed graphically. We identified several activated 'hotspot' regions harbouring a concentration of upregulated genes. Several 'hotspot' regions revealed integrin and Akt/NF-kappaB signalling. We identified key members linked to these signalling pathways including osteopontin (SPP1), glypican-3 (GPC3), annexin 2 (
ANXA2
), S100A10 and vimentin (VIM). Our integrative approach should significantly enhance the power of microarray data in identifying novel potential targets in human cancer.
...
PMID:Molecular mapping of human hepatocellular carcinoma provides deeper biological insight from genomic data. 1833 85
Annexins (ANXs) constitute a family of Ca2+-dependent membrane-binding proteins; at least 20 of them have been described to date. Among these,
Annexin A2
(
ANXA2
) has been revealed as a multi-functional protein in vitro. Its actual role in vivo, however, requires further investigation. We already reported that ANX-I (ANXA1) was up-regulated in
hepatocellular carcinoma
(
HCC
). The role of
ANXA2
in various liver diseases including
HCC
remains obscure. In the present study, the protein and mRNA levels of
ANXA2
, as well as its localization, were determined for the normal human liver, chronic hepatitis liver, and non-tumorous and tumorous portions of
HCC
tissues.
ANXA2
was rarely detected in either normal or chronic hepatitis liver tissues, whereas it was overexpressed at both the transcriptional and translational levels in tumorous and non-tumorous regions of
HCC
. In addition, in many cases, more
ANXA2
was expressed in the tumorous portion than in the non-tumorous portion of
HCC
. The expression of
ANXA2
was mainly localized in cancer cells, especially in poorly differentiated
HCC
. Furthermore,
ANXA2
was tyrosine-phosphorylated in
HCC
. These data suggest that overexpression and tyrosine phosphorylation of
ANXA2
play important roles in the malignant transformation process leading to
HCC
and are related to the histological grade of
HCC
.
...
PMID:Annexin A2 expression and phosphorylation are up-regulated in hepatocellular carcinoma. 1902 Jul 48
The development of
hepatocellular carcinoma
(
HCC
) is believed to be associated with multiple risk factors, including the infection of hepatitis B virus (HBV). Based on the analysis of individual genes, evidence has indicated the association between
HCC
and HBV and has also been expanded to epigenetic regulation, with an involvement of HBV in the DNA methylation of the promoter of cellular target genes leading to changes in their expression. Proteomic study has been widely used to map a comprehensive protein profile, which in turn could provide a better understanding of underlying mechanisms of disease onset. In the present study, we performed a proteomic profiling by using iTRAQ-coupled 2-D LC/MS-MS analysis to identify cellular genes down-regulated in HBV-producing HepG2.2.15 cells compared with HepG2 cells. A total of 15 proteins including S100A6 and
Annexin A2
were identified by our approach. The significance of these cellular proteins as target of HBV-mediated epigenetic regulation was supported by our validation assays, including their reactivation in cells treated with 5-aza-2'-deoxycytidine (a DNA methyltransferase inhibitor) by real-time RT-PCR and Western blot analysis, as well as the DNA methylation status analysis by bisulfite genome sequencing. Our approach provides a comprehensive analysis of cellular target proteins to HBV-mediated epigenetic regulation and further analysis should facilitate a better understanding of its involvement in
HCC
development.
...
PMID:iTRAQ-coupled 2-D LC-MS/MS analysis of protein profile associated with HBV-modulated DNA methylation. 1963 99
Annexin II
(
Annexin A2
,
ANXA2
) is a 36 kDa calcium-dependent phospholipid-binding protein that is located on the surface of most eukaryotic cells.
ANXA2
is involved in several biological processes, including anti-inflammatory effects, Ca27+-dependent exocytosis, immune responses, Ca2+ transport and phospholipase A2 regulation. In our previous study,
ANXA2
was identified as an up-regulated gene in
hepatocellular carcinoma
(
HCC
) tissue by cDNA microarray. In the present study, we have evaluated
ANXA2
as a tumor-associated marker of
HCC
. We determined the
ANXA2
levels in human liver tissues with
HCC
using real-time RT-PCR and Western blot analysis. For quantitative analysis of the
ANXA2 protein
in body fluids, we developed a sandwich ELISA system in which a polyclonal antibody and a monoclonal antibody specific to
ANXA2
were employed as a capture antibody and a probe antibody, respectively. We detected the
ANXA2
concentration in human serum using our newly developed system and evaluated its usefulness as a tumor marker. Overexpression of
ANXA2
in human liver tissue was confirmed by real-time RT-PCR and Western blot analysis. The sandwich ELISA system for
ANXA2
was developed for the detection of
ANXA2
in human samples. The dose-response relationship between
ANXA2
and optical density was linear in the range of 0-10 microg/ml and the sensitivity was 0.02 microg/ml. We determined the
ANXA2
concentration in serum specimens using the newly developed sandwich ELISA. The serum
ANXA2
concentrations of the patients with
HCC
(53.38+/-36.23 microg/ml) were significantly elevated when compared with those of normal individuals (28.81+/-24.94 microg/ml). These results suggest that expression of
ANXA2
may be increased in
HCC
patients and may play an important role in liver cancer progression. This new ELISA method can be used as a tool for the detection of
ANXA2
in human serum, particularly for cancer diagnostics.
...
PMID:Evaluation of annexin II as a potential serum marker for hepatocellular carcinoma using a developed sandwich ELISA method. 1988 16
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