Objective To evaluate the markers which contribute to diagnosis and prognosis of thyroid neoplasm. Methods The references about thyroid markers in recent years were reviewed. Results CD26 and galectin-3 could be regarded as a simple, potent markers to differentiate thyroid carcinoma in preoperative diagnosis, CD97 was a specific marker for undifferentiated thyroid carcinoma and its metastasis, CD15 and telomerase could be used in fine-needle aspirate biopsy (FNAB) of thyroid mass, and to improve its diagnostic evaluation, RET/PTC was mainly expressed in thyroid medullary carcinoma, oncofetal fibronectin (oncFN) was specific to papillary and anaplastic carcinoma, thyroid peroxidase was used to identify benign and malignant thyroid tumor. Conclusion Although there are a lot of markers for thyroid neoplasm, but there is no marker which are completely specific to certain histotype of thyroid neoplasm at present.
Objective To detect the anti-colon cancer ability of whole cell lysates pulsed dendritic cell (DC) which acts as an adjuvant. Methods Whole cell lysates of LoVo cells were extracted with freeze thawing method, then the monocyte-derived DC were pulsed with this cellular antigen. Subsequently, the capability of antigen pulsed DC to promote T lymphocytes proliferation and the ability of T lymphocytes to kill LoVo cells were detected by 3H-TdR incorporation and lactate dehydrogenase release methods, respectively. Results The whole cell lysates of LoVo cells pulsed DC significantly stimulated T cells proliferation, and the cytotoxicity abilities of primed T cells to kill LoVo cells were also enhanced. Conclusion Tumor cell lysates which act as the cellular antigen to pulse DC can improve the efficacy of anti-cancer immune response, which provides us an experimental evidence for cancer immunotherapy.
Objective To construct AWP1 (associated with protein kinase C related kinase 1) recombinant adenovirus as the tool of transferring the gene and investigate its expression and localization in human vascular endothelial cell ECV304. Methods Cloned AWP1 cDNA was inserted into the multiply clone sites (MCS) of plasmid pcDNA3 for adding flag tag, and the flag-AWP1 gene was subcloned into shuttle vector pAdTrack-CMV. After identified with restrictional enzymes, plasmid pAdTrack-flag-AWP1 was linearized by digestion with restriction endonuclease PmeⅠ, and subsequently cotransformed into E.coli BJ5183 cells with adenoviral backbone plasmid pAdEasy-1 to make homologous recombination. After linearized by PacⅠ, the homologous recombinant adenovirus plasmid transfected into 293 cells with Lipofectamine to pack recombinant adenovirus. After PCR assay of recombinant adenovirus granules, recombinant adenoviruses infected 293 cells repeatedly for obtaining the high-level adenoviruses solution. And then, the recombinant adenoviruses infected human ECV304 cells for observing the expression and localization of AWP1 under laser scanning confocal microscope (LSCM). Results PCR assay showed that recombinant adenovirus Ad-flag-AWP1 was obtained successfully; and ECV304 cells were infected high-efficiently by the homologous recombinant virus. Then, it was observed that flag-AWP1 protein expressed in ECV304 cells and distributed in the leading edges of the cell membrane. Conclusion The vectors of flag-AWP1 recombinant adenovirus are constructed, and the localization of AWP1 protein in ECV304 cells might show that AWP1 may be a potential role on the cell signal transduction.
Objective To evaluate the significance of serum colon cancer-specific antigen-2 (CCSA-2) in diagnosisof colorectal cancer (CRC). Methods By using ELISA method, the serum CCSA-2 was measured from 105 patients with 5 kinds of diseases, including CRC, gastric cancer, inguinal hernia, acute appendicitis, and breast cancer, who weretreated in our hospital from Jul. to Dec. in 2008, and 20 health donors were enrolled in addition. The blood samples were collected on 3 days before surgery, but blood samples from patients with acute appendicitis were collected before emergencysurgery, blood samples of health donors were collected on 1 day before ELISA test. Results The level of serum CCSA-2 in CRC patients was (99.27±6.25) μg/L, which was significantly higher than those of other patients and health individuals〔(53.58±2.73) μg/L, t=48.29, P=0.000〕. Serum CCSA-2 at a cutoff of 73.96μg/L had a sensitivity of 100% (95% CI:100%-100%) and a specificity of 100% (95% CI:100%-100%) in separating CRC populations from all other indivi-duals by using receiver operator characteristic curve (ROC) analysis. As compared with carcinoembryonic antigen (CEA) and CA19-9, the serum CCSA-2 assay (at a cutoff of 73.96μg/L) was significantly more sensitive than CEA and CA19-9 assay in CRC detection (P<0.01). Serum CCSA-2 was not related with patients’ gender (P=0.81), age (P=0.59), TNM stage (P=0.85), Dukes stage (P=0.63), nuclear grade (P=0.44), as well as expressions of multidrug resistance associated protein (P=0.33), P-glycoprotein (P=0.72), and topoisomeraseⅡ(P=0.95), but higher in patients with colon cancer than those of patients with rectal cancer (P=0.02). Conclusion Serum CCSA-2 may be a useful biomarker in diagnosis of CRC, and it may be only related to tumorigenesis, but is irrelated to tumor progression and chemotherapy.