1.Treatment of lumbar vertebral instability with posterior interbody fusion using autogenous bone and pedicle screw fixation
Qingyuan TAN ; Liming WANG ; Dongbo WANG
Orthopedic Journal of China 2006;0(05):-
[Objective] To investigate the clinical effect of treatment of lumbar vertebral instability with posterior interbody fusion using autogenous bone and pedicle screw fixation.[Methods]Thirty-seven cases of lumbar instability were treated with posterior spinal canal,nerve root canal decompression,pedicle screw fixation and autogenous bone grafting,and results were evaluated.[Results]Postoperative follow up time was average 25 months(ranged,12-32 months).Excellent fusion was achieved in 29 cases and good fusion was achieved in 8 cases,with good-to-excellent rate of 100%.According to JOA standard efficacy evaluation,postoperative JOA score improved significantly than preoperative one(P
2.ULTRASTRUCTURAL STUDIES ON THE GOAT OOGENESIS
Jinghe TAN ; Qingyuan SUN ; Zengming YANG ; Pengchun QIN
Acta Anatomica Sinica 1953;0(01):-
The cytoplasmic and nuclear changes during the development of goat oocytes were studied with light and electron microscopy. The oocyte development may be divided into 8 stages in accordance with the number and distribution of follicle cells and the size of the follicle. The results indicated that the Golgi complex, mitochondria, smooth endoplasmic reticulum and cortical granules became well developed and they moved into the cortical region as the oocyte development proceeded. In the oocytes in the follicle of 1.5-3mm in diameter, all the mitochondria became hooded and the number and size of fibrillar centers in the nucleolus reached maximum, but the nucleolar compaction still not occured at this stage. By the time when the follicle reached 3.5-5mm in diameter, the follicular cell processes began to degenerate, the microvilli of the oocyte withdrew from the zona pellueida and the oocytes might be cultured to mature in vitro. In the mature oocytes, Golgi complex and rough endoplasmic reticulum disappeared, the cortical granules arranged themselves in one layer beneath the oolemma, the mitochondria dispersed in the central region of cytoplasm and the eggs were ready for fertilization.
3.A comparative study of two reprogramming systems for inducing pluripotent stem cells from human dental origin
Xiaobing TAN ; Jingshu XU ; Guihu SUN ; Juncheng SONG ; Qingyuan DAI
Chongqing Medicine 2017;46(1):90-93
Objective To comparatively study the features of two reprogramming systems of induced pluripotent stem cells (iPSCs)from human dental origin.Methods Two kinds of reprogramming system,i.e.STEMCCA lentivirus /feed layer and Sen-dai virus /matrigel were used to induce human stem cells from apical papilla(SCAP)into iPSCs,respectively.The induction efficien-cies,workload of generating iPSCs,aneuploidy karyotype ratio,complexities of eliminating exogenous transcription factors and spe-cific markers expression were compared between these two systems.Results The STEMCCA reprogramming system required to prepare the feeder cell MEF.The reprogramming efficiency was 0.1%.Transcription gene-free iPSCs cells were obtained by the Cre-loxp enzyme digestion technique at the later stage.Sendai virus reprogramming system was feeder-free and the preparation of matrigel was quite simple with unified standard.The reprogramming efficiency was 0.7%,which was much higher than that of STEMCCA system(P <0.05).The exogenous virus and transgenes could be gradually eliminated after several passages of natural subclone.Conclusion The Sendai virus/matrigle reprogramming system is much more applicable for the induction of iPSCs from dental origin than the STEMCCA system.
4.Comparative characterization of osteo/odontogenic differentiation capability of human dental pulp stem cells and stem cells from apical papilla in vitro
Xiaobing TAN ; Yu GUO ; Jia LIU ; Jingshu XU ; Qingyuan DAI
Chongqing Medicine 2017;46(5):586-589
Objective To compare the growth characteristics,proliferation and osteo/odontogenic differentiation capability of stem cells from human dental pulp (dental pulp stem cells,DPSCs) and apical papilla (stem cells from apical papilla,SCAP) in vitro.Methods Human dental pulp and apical papilla tissues were separated from impacted third molars of young healthy donors at the age of root development and digested by collagenase type Ⅰ and dispase type Ⅱ to derive primitive DPSCs and SCAP.Cells were then induced for osteo/odontongenic differentiation by medium containing β-glycerophosphate,dexamethasone and KH2PO4.Flow cytometry was utilized to test the expression of specific markers of stem cells,including CD24,CD34,CD45,CD90,CD105,CD146,STRO-1 and OCT-4.AR-S was used to display the mineralization structure and RT-PCR was applied to analyze the expression of bone sialoprotein (BSP),osteocalcin (OCN) and dentine sialophosphoprotein (DSPP).Results Both DPSCs and SCAP were positive for CD90,CD105,CD146,STRO-1 and OCT-4,in percentages varying according to cell type,without expression of CD34 or CD45.Only SCAP expressed CD24 positively.Both cells formed organized mineralization structure after 2 weeks of induction in time-dependent manner,with more mineralization by SCAP and expressed differentiation markers,including BSP,OCN and DSPP.Conclusion Human DPSCs and SCAP possess the characteristics of MSCs and could be differentiated into odontonblast-like cells in vitro.Both cells are approachable stem cell sources for dental tissue engineering.
5.Comparison among 3 kinds of culture substrates of odontogenic induced pluripotent stem cells
Xiaobing TAN ; Jia LIU ; Yu GUO ; Jingshu XU ; Qingyuan DAI
Chongqing Medicine 2017;46(13):1743-1746
Objective To comparatively study the characteristics of 3 kinds of culture substrates of human odontogenic induced pluripotent stem cells(iPSCs).Methods The human odontogenic iPSCs were cultured by 3 kinds of substrates:mouse embryonic fibroblasts(MEF),matrigel and recombinant human vitronectin(VTN-N).The iPSCs growth situation was compared among three groups.Results The preparation time of these 3 kinds of substrates was 14,3,1 hlespectively,and,the difference was statistically significant (P<0.05).The iPSCs reprogramming time was (30± 1.6),(26 ± 2.1),(27 ± 1.4) d,lespectively,wht that in the MEF group significantly higer than in other two groups (P<0.05).The reprogramming efficiencies were 0.3 % ± 0.03 %,0.56 % ± 0.08 %,0.7 % ± 0.02 % respectively (P< 0.05).Three kinds of substrate could better support iPSCs growth and make them to maintain un-differentiation status.Conclusion with no heterologous animal components,and the adrantaga of simple pleparation,oonfrollable standard and shorter gramming time is easy to prepare,the standard is controllable and the reprogramming time is shorter,which is an ideal substrate for supporting iPSCs growth.
6.Experimental study on the curative effect of Huoxue-Tongluo-Zhitong ointment treating acute soft issue injury
Liming WANG ; Qingyuan TAN ; Yan ZHANG ; Guanjun QIU ; Hongxue QU ; Weidong ZHANG
International Journal of Traditional Chinese Medicine 2011;33(10):893-896
Objective To observe the curative effect of Huoxue-Tongluo-Zhitong ointment treating soft tissue injury,and the safety of application on skin.Methods The treatment group was treated with Huoxue-Tongluo-Zhitong ointment,while the comparison group was treated with Votalin Pill.Acute toxicity experiment,irritant experiment and hypersensitivity experiment of skin were performed on New Zealand white rabbits.Results Huoxue-Tongluo-Zhitong ointment decreased local edema and leukocyte effusion,accelerate the re-absorption of hematomas.On injury signs index,group A [ (0.32± 0.35),(0.29± 0.27) ] was better than group B [ (0.58±0.42),(0.91 ±0.34) ] (P<0.05).The pathological process in group A and B was obviously reduced than group C (P<0.05).In the neutruphil infiltration density measuring:compared with group C,group A and B both showed significant difference (P<0.05),but there was no significant difference between group A and B (P>0.05).Conclusion Huoxue-Tongluo-Zhitong ointment performed well on the treatment of soft issue injury,with no toxicity,irritation,and hypersensitivity of skin,as well as high safety of administration.
7.Course construction and practice of progress in pathophysiology for postgraduate students
Junze LIU ; Qingyuan HUANG ; Gang ZHANG ; Wenxiang GAO ; Xiaoling TAN ; Weigong LIAO ; Youming FAN ; Mingchun CAI ; Jian CHEN
Chinese Journal of Medical Education Research 2012;11(1):25-28
Proceeding from the requirements of teaching target for postgraduate students,the course of progress in pathophysiology was constructed and administrated.The course objective was defined which combined teaching knowledge with fostering students' ability together,especially the ability to think new ideas and to do scientific research.Aiming at this teaching target,the teaching contents which combined with the direction of scientific research of the department was growing together with scientific development,especially in new knowledge and new technique.Multiple teaching means and several mode of examine were adopted during the process of teaching practice.
8. Correlation between fetal cranial nervous system malformation and chromosome abnormality
Xiaolei XIE ; Fuguang LI ; Weihe TAN ; Suhuan TANG ; Jiang TANG ; Li WANG ; Dandan WANG
Chinese Journal of Applied Clinical Pediatrics 2019;34(21):1649-1652
Objective:
To investigate the correlation between fetal cranial nervous system malformation and chromosome abnormality.
Methods:
The pregnant women with fetal cerebral nervous system dysplasia were collected from January 2013 to August 2018 at the Prenatal Diagnostic Center of the Sixth Affiliated Hospital of Guangzhou Medical University.The fetus was diagnosed by ultrasonography and karyotype analysis.
Results:
A total of 18 cases of abnormal karyotypes were detected from 85 patient samples, and the abnormal rates were 21.18%.Single cranial nervous system malformation was found in 47 cases, abnormal karyotypes in 4 cases, multiple system malformation in 38 cases, and abnormal karyotypes in 14 cases, and the abnormal karyotype rate of multiple system malformation was higher than that of single cranial nervous malformation (36.84%
9.Prenatal diagnosis of a fetus with trisomies of 11q23.3q25 and 22q11.1q11.21.
Fuguang LI ; Jiang TANG ; Xiaojie XIE ; Suhuan TANG ; Aijian WU ; Qiaomin TANG ; Weihe TAN ; Xiaoyan GUO
Chinese Journal of Medical Genetics 2019;36(6):632-635
OBJECTIVE:
To explore the phenotype and pathogenesis of a fetus with a rare chromosomal abnormality.
METHODS:
The fetus was analyzed by clinical prenatal ultrasonography, G-banding karyotyping and next generation sequencing (NGS).
RESULTS:
Prenatal ultrasonography of the fetus showed Dandy-Walker syndrome, growth restriction, and right-heart system dysplasia. The fetus had a chromosomal karyotype of 47,XY,t(11;22)(q23.3;q11.2),+der(22)t(11;22). Duplication of 11q23.3q25 and 22q11.1q21 were also detected by NGS. The chromosomal translocation carried by the fetus was derived from his father.
CONCLUSION
Duplications of chromosome 11q23.3q25 and 22q11.1q11.21 segments probably underlie the Dandy-Walker syndrome, growth restriction, and hypoplasia of the right heart system in the fetus.
Chromosome Disorders
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Chromosomes, Human
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Female
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Fetus
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Humans
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Karyotyping
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Pregnancy
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Prenatal Diagnosis
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Translocation, Genetic
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Trisomy
10.Characterization of microRNAs profiles of induced pluripotent stem cells reprogrammed from human dental pulp stem cells and stem cells from apical papilla.
West China Journal of Stomatology 2017;35(3):269-274
OBJECTIVETo compare characterization of microRNAs (miRNAs) expression profiles of induced pluripotent stem cells (iPSCs) reprogrammed from human dental pulp stem cells (DPSCs) and stem cells from apical papilla (SCAP) and screen-specific microRNA.
METHODSHuman DPSCs and SCAP were reprogrammed into iPSCs using a Sendai virus vector. Total RNA of human DPSCs-iPSCs and SCAP-iPSCs were extracted. miRNAs were labeled and hybridized. Slides were scanned, and images were imported into GenePix Pro 6.0 for grid alignment and data extraction. Significant differentially expressed miRNAs between the two groups were identified using fold change and P-value and were analyzed.
RESULTSBoth human DPSCs and SCAP were successfully reprogrammed into iPSCs. Among miRNA genes analyzed by miRNA microarray, 68 were differentially expressed by more than 10-fold in DPSCs-iPSCs; 37 of these genes were up-regulated, and 31 were down-regulated. In SCAP-iPSCs, 107 genes were differentially expressed by more than 10-fold; 68 were up-regulated, and 39 were down-regulated. In both cells, only miR-302e was up-regulated, whereas 9 miRNAs were down-regulated: miR-29b-3p, miR-181b-5p, miR-4328, miR-22-5p, miR-145-5p, miR-4324, let-7b-5p, miR-181a-5p, and miR-27b-3p.
CONCLUSIONSMultiple miRNAs participated in reprogramming of human DPSCs and SCAP into iPSCs. Most miRNAs are related to cell cycle, transforming growth factor-β signaling pathways and epithelial-mesenchymal transition.
Cell Cycle ; Cell Division ; Dental Pulp ; Down-Regulation ; Electrodes ; Epithelial Cells ; Humans ; Induced Pluripotent Stem Cells ; MicroRNAs ; Taste Buds ; Up-Regulation