PMID- 12378620
OWN - NLM
STAT- MEDLINE
DCOM- 20030211
LR  - 20190430
IS  - 1007-9327 (Print)
IS  - 2219-2840 (Electronic)
IS  - 1007-9327 (Linking)
VI  - 8
IP  - 5
DP  - 2002 Oct
TI  - Preparation of monoclonal antibody against apoptosis-associated antigens of 
      hepatoma cells by subtractive immunization.
PG  - 808-14
AB  - AIM: To elucidate the expression of the apoptosis-associated molecules in human 
      primary hepatocellular carcinoma (HCC) cells, and prepare the monoclonal 
      antibodies (mAb) against the apoptosis-associated antigens of HCC cells. METHODS: 
      Human HCC cell line HCC-9204 cells were induced apoptosis with 60 mL x L(-1) 
      ethanol for 6 h and their morphological changes were observed by transmission 
      electron microscope. The cell DNA fragmentations were detected by Terminal 
      Deoxynucleotidyl transferase-mediated dUTP nick end labeling (TUNEL) assay, and 
      the cell DNA contents by flow cytometry. Ten mice were immunized with 
      ethanol-induced apoptotic HCC-9204 cells with the method of subtractive 
      immunization, while the other 10 mice used as the control were immunized by the 
      routine procedures. The tail blood of all the mice were prepared after the last 
      immunization, and the produced antibodies were determined by the 
      immunocytochemical ABC staining. The splenic cells of the mice whose tail blood 
      sera-HCC-9204 cells serum reactions were most different between the apoptotic and 
      the non-apoptotic were prepared and fused with the mouse myeloma cell line SP2/0 
      cells. The positive antibodies were selected by ELISA assay. The fusion rates of 
      hybridoma cells and the producing rates of antibodies were calculated. The fused 
      cells that secreted candidate objective antibody were cloned continually with the 
      of limited dilution method, and then selected and analyzed further by the 
      immunocytochemical ABC staining. The chromosomes of the cloned hybridoma cells 
      that secreted objective mAb and the mAb immunoglobulin (Ig) subtype of the 
      prepared mAb were also determined. The molecular mass of the mAb associated 
      antigen was analyzed by Western blot assay. RESULTS: HCC-9204 cells treated with 
      60 mL x L(-1) ethanol for 6 h, manifested obvious apoptotic morphological 
      changes, the majority of the cells were TUNEL-positive, and the sub-G1 apoptotic 
      peak was evident. There were 2 mice in the experimental group whose tail blood 
      serum reacted strongly with the apoptotic HCC-9204 cells, but weakly with their 
      non-apoptotic counterparts. In the fusion rates of hybridoma cells as well as the 
      producing rates of the antibody described above, there did not show significant 
      difference between the experimental and the control group, but weakly with 
      non-apoptotic HCC-9204. However, the total producing rate of antibodies in the 
      experimental group was significantly lower compared with the control (P<0.01), 
      and so was the producing rate of the antibodies which reacted strongly with both 
      apoptotic and non-apoptotic HCC-9204 cells(P<0.01). After cloned continually for 
      several times the cell that produce mAb which reacted strongly with the nuclei of 
      ethanol-induced apoptotic HCC-9204 cells, but very weakly with that of 
      non-apoptotic cells was selected out. Chromosome analysis revealed that the 
      selected cell was with the universal characteristics of the monoclonal hybridoma 
      cells which secreted mAb, and the Ig subtype of the prepared mAb was IgG1. The 
      molecular mass of this mAb associated antigen of was about 75 ku. CONCLUSION: 
      Subtractive immunization is a useful method to prepare the mAb against the 
      apoptosis-associated antigens of cells. The expression of some molecules 
      increases to some extent in HCC-9204 cells in the process of apoptosis induced by 
      low-concentration ethanol. The mAb that may be against ethanol-induced 
      apoptosis-associated antigens of HCC cells was successfully prepared and 
      primarily identified.
FAU - Yang, Lian-Jun
AU  - Yang LJ
AD  - Department of Pathology, Institute of Cancer Research, The Fourth Military 
      Medical University, Xi'an 710032, Shaanxi Province, China.
FAU - Wang, Wen-Liang
AU  - Wang WL
LA  - eng
PT  - Journal Article
PT  - Research Support, Non-U.S. Gov't
PL  - United States
TA  - World J Gastroenterol
JT  - World journal of gastroenterology
JID - 100883448
RN  - 0 (Antibodies, Monoclonal)
RN  - 0 (Antigens, Neoplasm)
RN  - 0 (DNA, Neoplasm)
RN  - 0 (Immunoglobulin G)
SB  - IM
MH  - Antibodies, Monoclonal/*immunology
MH  - Antigens, Neoplasm/chemistry/*immunology
MH  - Apoptosis/*immunology
MH  - *Carcinoma, Hepatocellular
MH  - Cell Fusion
MH  - DNA, Neoplasm/analysis
MH  - Humans
MH  - Hybridomas
MH  - Immunization
MH  - Immunoglobulin G/immunology
MH  - *Liver Neoplasms
MH  - Microscopy, Electron
MH  - Molecular Weight
MH  - Tumor Cells, Cultured/immunology/ultrastructure
PMC - PMC4656566
EDAT- 2002/10/16 04:00
MHDA- 2003/02/13 04:00
PMCR- 2002/10/15
CRDT- 2002/10/16 04:00
PHST- 2002/10/16 04:00 [pubmed]
PHST- 2003/02/13 04:00 [medline]
PHST- 2002/10/16 04:00 [entrez]
PHST- 2002/10/15 00:00 [pmc-release]
AID - 10.3748/wjg.v8.i5.808 [doi]
PST - ppublish
SO  - World J Gastroenterol. 2002 Oct;8(5):808-14. doi: 10.3748/wjg.v8.i5.808.