Experimental establishment of in situ and subcutaneous transplantation models of human liver malignant lymphoma in nude mice
Experimental establishment of in situ and subcutaneous transplantation models of human liver malignant lymphoma in nude mice
The establishment of in situ and subcutaneous transplantation models of human hepatic malignant lymphoma in nude mice can (1) explore the pathogenesis of hepatic malignant lymphoma, (2) provide a tool for experimental therapies, and (3) provide tumor animal models for experimental studies on the etiology and pathogenesis of hepatic malignant lymphoma.
Operation method
In situ and subcutaneous graft models
Principle
Human liver malignant lymphoma was implanted into the liver parenchyma and interscapular subcutis of nude mice with fresh tissue blocks from the operation to observe the tumorigenicity rate of in situ transplantation and subcutaneous transplantation, invasion and metastasis of the transplanted tumors, and to perform morphological (light microscopy, electron microscopy, immunohistochemistry), serological [alpha-fetoprotein (AFP), Hepatitis B Virus Surface Antigen (H BsAg), lactic acid dehydrogenase (LDH)], karyotypic and flow cytometric analyses. Karyotype and flow cytometric analysis.
Materials and Instruments
BALB C-nu nu nude mice Fresh specimen of liver malignant lymphoma Move I. Preparation of experimental animals Caveat It is because the liver microenvironment of nude mice is similar to that of human liverThe similarity of the implanted tumors to human liver provides an ideal animal model for basic and clinical studies of primary malignant lymphoma of the liver, as the implanted tumors appear to be similar to the dissemination process of human liver primary malignant lymphoma. Common Problems For more product details, please visit Aladdin Scientific website.
RPMI-1640 culture medium Tincture of iodine Alcohol Sodium pentobarbital CD3 antibody CD7 antibody CD19 antibody CD20 antibody CD45RO antibody CD79a antibody
Silk thread Optical microscope Casing needle Scalpel Gauze
BALB/C-nu/nu nude mice, aged 4~6 weeks, weighing 17~20 g, both male and female, were reared under specific-pathogen free (SPF) conditions in the nude mouse room of our hospital.
Sources of specimens
1. The fresh specimen of hepatic malignant lymphoma came from a 53-year-old male patient, whose preoperative laboratory tests were normal for liver function, AFP, CEA, and bone marrow image, except for elevated LDH (1,200 U/L) and positive HBsAg. 2.
2. The operation confirmed multiple nodular lymphoma of the liver, with multiple nodules in the right lobe of the liver and multiple nodules in the left lobe fused into a 5.3 cm x 3.5 cm x 3.0 cm mass, which was grayish-white and fish-like in color, with yellowish-white in the middle of the nodule and red irregular congested bands in the periphery.
3. There was no other tissue or organ invasion or involvement of distant lymph nodes during the operation, and the pathological diagnosis of the tumor nodule in the left lobe of the liver was non-Hodgkin's B-cell-derived malignant lymphoma of the liver and chronic hepatitis.
Specimen processing
Aseptically cut human liver malignant lymphoma biopsy, put into RPMI-1640 culture solution, remove the non-tumor tissue, and cut it into 1 mm x 1 mm x 1 mm tissue pieces for transplantation.
Subcutaneous transplantation
The skin on the back of nude mice was sterilized with 2.5% tincture of iodine and 75% alcohol, and two 1 mm x 1 mm x 1 mm lumps of tumor tissue were aspirated with a sterile cannula needle and transplanted into the subcutaneous tissue on the back of the neck.
V. In situ transplantation
1. Nude mice were anesthetized with sodium pentobarbital (30 mg/kg) intravenously, a transverse incision was made in the left upper abdomen to expose the liver, the peritoneum of the left lobe of the liver was incised, and two 1 mm x 1 mm x 1 mm tumor blocks were implanted into the hepatic parenchyma. The hepatic peritoneum was closed by 10-0 nondestructive threads, the peritoneum was closed by 7-0 threads, and the skin was sewn up by 5-0 threads.
2. After the operation, we continued to feed and observe the growth of the tumor day by day.
Transmission
1. When the tumor-bearing nude mice are in a state of near-death, take one of the tumor-bearing nude mice and execute it by cervical dislocation, systematically dissect it and take out the transplanted tumor. 2.
2. One part of the transplanted tumor tissue will be transmitted to the other mice by the method of primary transplantation, with 5~10 nude mice each time; the other part of the tumor tissue will be frozen in liquid nitrogen for spare use, and will be used for the detection of relevant indexes. 3.
3. The other tumor-bearing nude mice were kept until near death or natural death to observe the growth, invasion and metastasis of the tumors.
VII. Observation Items
1. Anatomical and histological examination
(1) All executed and naturally dead nude mice with tumor were subjected to detailed anatomical examination, and the growth of intrahepatic tumors and subcutaneous graft tumors were recorded.
(2) Lymph nodes were sampled from the para-iliac arteries, inter-iliac arteries, mediastinum, mesentery, pylorus, cardia and hepatic hilar lymph nodes, etc. Organs such as lungs, livers, spleens, kidneys, brains and other organs were routinely sampled, and all the tissues were fixed with 10% neutral formaldehyde, paraffin sections were cut, stained with hematoxylin, eosin and light microscopy was carried out.
2. Immunohistochemical staining
Immunohistochemical staining was performed on all liver tumor sections of nude mice with CD3, CD7, CD19, CD20, CD45RO, CD79a antibodies using LSAB method.The reagents used were purchased from DaKo Company.
3. Electron microscopic observation
The transplanted tumors were double-fixed with 2.5% glutaraldehyde and 1% osmium acid, embedded in Epon-812, ultrathin sectioned, stained with uranium and lead, and observed by transmission electron microscope with PHILIPS-CM10.
4. Laboratory tests
AFP immunoassay; Hepatitis B markers: HBsAg, HBeAg, HBsAb, HBeAb, HBcAgELISA; LDH-L method.
5. Flow cytometry analysis
Flow cytometer (FACS-420) was used to measure the DNA content of normal hepatocytes, tumor-derived specimens and transplanted tumor cells.
6. Chromosome examination
The cells were cultured for a short period of time without mitotic stimulation, and the harvested cells were prepared routinely, stained with GTG method and observed under the microscope.
7. Histologic classification of malignant lymphoma.
The new WHO classification of 2001 should be adopted.
8. Statistical treatment
The significance of differences was determined by t-test, and the data were expressed as x±s, which was done on SPSS 10. 0 statistical software.
Reference Zhang N, Tuo Shuai, Liu Qiu Zhen et al. Establishment and biological characterization of in situ and subcutaneous transplantation models of human liver malignant lymphoma in nude mice. Digestive Surgery , 2006 (5)
