LB was performed
when no conclusion could be drawn from the non-invasive work up. Etiology of chronic hepatitis at our centre, hepatitis B (HBV) 66 %, hepatitis C (HCV) 17% Autoimmune 7.5%, while cryptogenic 1.6%. Etiology of cirrhosis was alcoholic 32%, HBV 19%, HCV 14% and autoimmune 6.3%, cryptogenic 18%. Etiology of acute liver disease was as follows: Hepatitis A 9%, HBE 37%, HBV 8 %, and drugs 6.9%. Out of these 3,000 patients LB was done on 176 patients (5.86%, male 116, age 20–65 years) LB was performed with biopsy gun under ultrasound guidance. Patients with platelet count <50,000, with ascites and overt bleeding were excluded. Patients were not excluded even INR >1.5. No prophylactic use of fresh frozen plasma and platelet transfusion was done. 38 patients (21.5%) had platelet count ranging from 50,000 to l,00,000. Roxadustat mouse 28 patients (16%) had prothrombin time (PT) INR > 1.5 (range 1.6–4). There was no major complication related to the procedure. Indications for LB were as follows : Autoimmune hepatitis 30, cryptogenic LD 38, drug induced LD 4, evaluation of portal hypertension 15, mass lesion in the liver and lymphoma 29, elevated HM781-36B manufacturer liver enzymes
11, hepatitis B infection 35, hepatitis C infection 9, other miscellaneous indications were Primary biliary cirrhosis, primary sclerosing cholangitis, drug induced liver injury, sepsis related cholestasis, sarcoidosis, amyloidosis etc. Results: LB changed the diagnosis in 55(27%). Patients in this category were evaluation of portal hypertension 15, elevated liver enzymes 11, cryptogenic 24 and other diagnosis were cholestatic liver disease, amyloidosis and myeloproliferative disorders. In remaining VAV2 patients LB confirmed clinical diagnosis and helped in making management decisions Conclusion: 5–6% patients with LD need biopsy. LB is safe even in presence of low platelet count and abnormal INR. 1/4th of the patients undergoing LB change the clinical diagnosis. Key Word(s): 1. Autoimmune;
2. Cryptogenic; 3. amyloidosis; 4. granuloma; Presenting Author: LIN TAO Additional Authors: HAIXING JIANG, QUNXIN JIN, SHIJIA MA Corresponding Author: HAIXING JIANG, QUNXIN JIN Affiliations: First Affilated Hospital of Guangxi Medical University Objective: To observe the process of collecting, transfering species and purifying and passaging of Blastocystis hominis. To determinate the organelle marker enzyme in B.hominis, then provide stable insect strains and research base for further study of morphology and function of B.hominis Methods: Concentraed B.hominis strains via Aldehyde-ether method. DMEM medium was used to cultured B.hominis in vitro, and observed the biological characteristics; determinated MTT colorimetry OD value of the growth curve; determinated of the organelle marker enzyme of B.hominis by electron microscopic enzyme cytochemical method. Results: 1. B.hominis is adherent growth. Passaged B.