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find Author "周红雨" 14 results
  • Bedside Assessment of Swallow in Stroke

    摘要:目的:探索可靠的卒中患者床旁吞咽评估方法。方法:61例住院卒中患者均进行各种床旁吞咽评估筛查及电视透视检查,以后者为金标准探讨各方法的敏感度、特异度及阳性、阴性预测值。结果:六种独立床旁吞咽评估方法与金标准相比较的敏感度在60%~87%之间,特异度在76%~89%之间,阳性预测值在50%~69%之间,阴性预测值在86%~95%之间;几种评估方法作为平行试验联合应用时的敏感度在89%~98%之间,阴性预测值在94%~99%之间;几种方法作为序列试验应用时的特异度在97%~99%之间,阳性预测值在82%~90%之间。结论:根据不同方法的预测特点,可得到针对不同患者的、有效的床旁评估方法。床旁吞咽评估简单、有效、便捷,是临床工作中适宜的评估方法。

    Release date:2016-08-26 03:57 Export PDF Favorites Scan
  • EXPERIMENTAL STUDY ON MICRO-DYSTROPHIN GENE TRANSFECTION INTO C57/BL10 MICE’S MYOBLAST

    Objective To investigate the expression of micro-dystrophin gene in myoblast cultured in vitro, to explore the possibil ity of combining myoblast transplantation with gene transfer for Duchenne muscular dystrophy therapy. Methods Competent Escherichia coli JM109 was prepared, which transformed with plasmid pSL139, and positive clones were picked to cultivate. Plasmid was extracted with Alkal ine lysis method and cutted with both Pvu I and Cla I enzyme. Agarose gel electrophoresis was employed to take pictures. Ten healthy 5-7 days old male C57/BL10 mice were selected, weighing4-5 g, the primary and subcultured myoblasts were cultured with multi-step enzymatic digestion and differential adhesionmethod, and Desmin immunofluorescent method was used to identfy. The 3rd generation myoblasts that were transfected with plasmid pSL139 mediated by l iposome served as the experimental group, untransfected cells served as the control group. After 48 hours of transfection, the expressions of micro-dystrophin mRNA and protein in myoblasts were detected with RTPCR and cell immunofluorescent methods, and the transfection efficiency was caculated. Results After pSL139 plasmids being digested and for 40 minutes agarose gel of electrophoresis, 3.75 kb fragment of target gene and vector were observed. The cells were almost uniform, and triangular or diamond shape after 24-48 hours of culture; the cells turned to fusion manner and could be passaged after 4-6 days. Desmin immunofluorescent result showed that green fluorescence was seen in cytoplasm of most 2nd myoblasts, and the purity of the myoblasts was above 90%. At 48 hours after transfection of myoblasts with plasmid pSL139, RT- PCR results showed that about 300 bp fragment was seen in the experimental group and the control group, and the brightness was higher in experimental group. Immunofluorescent staining displayed that green fluorescence was seen in the cytoplasm of the myoblasts in the experimental group and no green fluorescence in the control group; the expression efficiency of positive cells for micro-dystrophin was 45%-55% in experimental group. Conclusion Micro-dystrophin gene can highly express at the levels of mRNA and protein respectively in myoblasts transfected with plasmid pSL139 mediated by l iposome.

    Release date:2016-08-31 05:48 Export PDF Favorites Scan
  • EXPERIMENTAL STUDY OF TREATING DUCHENNE MUSCULAR DYSTROPHY WITH MYOBLAST TRANSPLANTATION

    Objective To investigate the effect of myoblast transplantation on duchenne muscular dystrophy (DMD) and to explore the method and feasibil ity of applying gene therapy to DMD. Methods Myoblast of C57/BL10 mice were cultured using multiple-step enzyme digestion method and differential velocity adherent technique. The morphology of the cells was observed with inverted phase contrast microscope. The cells at passage 4 were labeled with 5-BrdU. Twenty-four DMDmodel mice (mdx mice: aged 4-6 weeks, male, 13.8-24.6 g) were randomly divided into two groups (n=12 per group): group A, 1 × 106/mL labeled myoblast were injected via ven caudal is twice at an interval of 2 weeks; group B: 1 mL DMEM/F12 was injected in the same manner serving as a control group. The mice were killed 4 weeks after operation and the motor abil ity of the mice was detected by one-time exhaustive swimming before their death. HE staining and immunohistochemistry staining observation for 5-BrdU, desmin, and dystrophin (Dys) were preformed, and the imaging analysis was conducted. Results The primary myoblast could be sub-cultured 5-7 days after culture, providing stable passage and sufficient cells. The time of onetime exhaustive swimming was (60.72 ± 5.76) minutes in group A and (47.77 ± 5.40) minutes in group B, there was significant significance between two groups (P lt; 0.01). At 4 weeks after injection, HE staining showed that in group A, there were round and transparent-stained myocytes and the percentage of centrally nucleated fibers (CNF) was 67%; while in group B, there were uneven muscle fiber with such pathological changes as hypertrophia, atrophia, degeneration, and necrosis, and the percentage of CNF was above 80%. Immunohistochemistry staining revealed that the expression of 5-BrdU, desmin, and Dys was positive in group A; while in group B, those expressions were l ittle or negative. Image analysis result displayed that integral absorbency (IA) value of desmin was 489.70 ± 451.83 in group A and 71.15 ± 61.14 in group B (P lt; 0.05) and the ratio of positive area to thetotal vision area was 0.314 3 ± 0.197 3 in group A and 0.102 8 ± 0.062 8 in group B (P lt; 0.05); the Dys IA value was 5 424.64 ± 2 658.01 in group A and 902.12 ± 593.51 in group B (P gt; 0.05) and the ratio of positive area to the total vision area was 0.323 7 ± 0.117 7 in group A and 0.035 2 ± 0.032 9 in group B (P lt; 0.05). Conclusion Myoblast transplantation has certain therapeutic effect on DMD of mice.

    Release date:2016-09-01 09:08 Export PDF Favorites Scan
  • PRESENT AND FUTURE OF CLINICAL APPLICATION OF MYOBLAST

    Objective To introduce the current situation and futureof myoblast transfer therapy (MTT) in clinical application Methods The latest fifteenyear literatures were extensively reviewed, concerninggene therapy for Duchenne’s muscular dystrophy, Parkinson’s disease, myelopathy, permanent facial paralysis, angiocardiopathy, injuries of bone, joint and muscle, hematopathy, and pituitary dwarf. Results In medical field, MTT is an ideal method to treat some common diseases. The problems were immunologic rejection and better carriers for myoblasts implantation. Conclusion It is the focus on the use of myoblast as a vector to carry exogenous gene in some disease therapy. The major problems of MTT include transplantation immunity, cell fusion and target protein expression. It is easy to gain,culture and transfuse to the host for myoblasts, these merits are beneficial to clinical application. 

    Release date:2016-09-01 09:23 Export PDF Favorites Scan
  • Initial Analysis of Correlation Factors of Leukoaraiosis

    目的:探讨单纯脑白质疏松症(LA)以及LA合并脑梗死及其MRI影像学严重程度与年龄、性别、高血压、糖尿病相关性初步分析。方法:根据郭氏等2003年制定的LA诊断标准纳入168例脑白质疏松症患者,分为A、B两组:A组95例为单纯脑白质疏松(LA),B组73例为LA合并脑梗死(LA+CI)。两组患者均行头MRI检查。根据Kinkel等的方法将T2WI显示脑室周围高信号范围及程度分为5型.结果:年龄与脑白质疏松的严重程度呈线性相关性(Plt;0.05),男性与女性间比较脑白质疏松的发生率无显著差异(Pgt;0.05),LA以及LA+CI患者,其高血压及糖尿病伴发率较高,而且LA+CI组高于LA组(高血压Plt;0.01,糖尿病Plt;0.01),LA患者MRI表现以1型为主,LA+CI患者表现以2型为主,Plt;0.01)。结论:脑白质疏松症的严重程度与年龄密切相关,LA的发生率在男女性别间无明显差异。高血压、糖尿病可能是LA的危险因素。LA+CI组与单纯LA组相比,其高血压、糖尿病伴发率更高且MRI表现程度更重。

    Release date:2016-09-08 09:54 Export PDF Favorites Scan
  • 视神经脊髓炎谱系疾病合并重症肌无力、干燥综合征及桥本甲状腺炎首例报告

    Release date:2018-03-07 04:35 Export PDF Favorites Scan
  • Clinical Features of Neuromyelitis Optica Combined with Abnormal Immune Parameters

    【摘要】 目的 分析合并免疫指标异常的视神经脊髓炎临床特点。 方法 回顾性分析2009年5月-2010年11月收治的62例视神经脊髓炎患者中24例合并免疫指标异常患者的临床资料。24例均为女性,发病年龄14~53岁。对其临床表现、视觉诱发电位、影像学检查结果、免疫检查结果进行分析。 结果 所有患者均有脊髓和视神经同时或先后受累的表现。24例视觉诱发电位检查23例异常。脊髓MRI显示病变集中于颈段、上胸段脊髓。颈段和胸段脊髓同时受累17例,单纯颈段脊髓受损6例,单纯胸段脊髓受损1例。所有患者抗核抗体滴度均≥1∶100,合并抗SSA抗体阳性14例(55.5%),同时合并抗SSB抗体阳性11例(45.8%),合并抗Rib抗体阳性1例,合并抗SCL-70抗体阳性1例,合并抗dsDNA抗体1例。 结论 视神经脊髓炎合并免疫指标异常的患者以女性较为多见,易复发,青壮年患者发病率最高。脊髓MRI示病变集中于颈段、上胸段脊髓,表现为长节段脊髓损害。视神经脊髓炎患者合并结缔组织病的病例较多。【Abstract】 Objective To analyze the clinical features of neuromyelitis optica (NMO) combined with abnormal immune parameters. Methods We retrospectively reviewed the clinical data of 24 patients with NMO and abnormal immune parameters among the 62 NMO patients who were admitted into our department between May 2009 and November 2010. All patients were female, aged from 14 to 53 years. We analyzed their clinical manifestations, visual evoked potentials, imaging results, and immunological examinations. Results All patients had simultaneous or successive spinal cord and optic nerve involvement. Twenty-three patients had abnormal visual evoked potential. MRI showed that the lesions focused on the cervical and upper thoracic spinal cord. Both cervical and thoracic spinal cord were involved in 17 cases; there were 6 cases of simple cervical spinal cord injury and 1 case of simple thoracic spinal cord damage. Antinuclear antibody titer of all the patients was ≥1∶100. Combined positive anti-SSA antibody occurred in 14 patients (55.5%); Concomitant positive anti-SSB antibodies occurred in 11 patients (45.8%); Combined positive anti-Rib antibodies occurred in 1 patient; Combined positive anti-SCL-70 antibody occurred in 1 patient; and combined positive anti-dsDNA antibodies occurred in 1 patient. Conclusions NMO combined with abnormal immune parameters mainly occurs in female patients, especially in young people. Recurrence rate is high. MRI shows that the lesions focus mainly on the cervical and upper thoracic spinal cord, manifesting the characteristic of long segment damage. And NMO is frequently combined with connective tissue disease.

    Release date:2016-09-08 09:27 Export PDF Favorites Scan
  • 氯化钾加入甘露醇治疗低钾型周期性麻痹42例疗效观察

    目的:探讨更为安全、有效的静脉补钾治疗低钾型周期性麻痹的方法。方法:收集本院住院低钾型周期性麻痹患者,应用半随机法分为治疗组和对照组进行临床对照研究。治疗组将氯化钾加入5%甘露醇静脉补钾,对照组常规补钾,监测血钾及肌力的恢复情况。结果:治疗组疗效明显,优于对照组(Plt;0.05)。结论:将氯化钾加入5%甘露醇治疗低钾型周期性麻痹疗效好,安全可行。

    Release date:2016-09-08 09:54 Export PDF Favorites Scan
  • 基于雨课堂的翻转课堂模式在长程脑电图教学实践中的探索

    长程脑电图(Long-term electroencephalogram,LT-EEG)教学是神经专科教学的重要组成部分,其专业性强,理论抽象,图形复杂,学生学习难度大,传统的教学模式难以理解和掌握。翻转课堂作为一种新型的教学模式,能够有效提高学生的学习主动性和参与度。雨课堂作为一款智慧教学平台已被各大高校应用于多种教学领域。本文探讨了基于雨课堂平台的翻转课堂模式在 LT-EEG教学的应用实践。通过详细描述教学设计、实施过程及效果评估,本文旨在探索如何利用雨课堂平台以及优化长程脑电图的教学效果,提升学生的学习效果和实践能力,激发学员学习兴趣,提高脑电图教学质量,促进学科的应用和发展,为神经专科和相关专业培养合格医疗人才奠定坚实的基础。

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  • EXPERIMENTAL STUDY ON EFFECT OF MONOCYTE CHEMOATTRACTANT PROTEIN 1 ON MIGRATION OF INDUCED AND DIFFERENTIATED MOUSE BONE MARROW MESENCHYMAL STEM CELLS IN VITRO

    Objective To investigate the effect of monocyte chemoattractant protein 1 (MCP-1) on the migration of the induced and differentiated mouse bone marrow mesenchymal stem cells (BMSCs) for raising the efficacy of intravenous transplantation of BMSCs. Methods The BMSCs were cultured with the method of differential adhesion and density gradient centrifugation of C57/BL10 mice, and were identified by alkal ine phosphatase Gomori modified staining after osteogenic inducing. At the 3rd passage, the BMSCs were induced to the myoblasts with 5-azacytidine (5-Aza). The chemotaxis of MCP-1 in the induced and differentiated BMSCs in vitro at concentrations of 25, 50, 100, 200, and 400 ng/mL was observed through the migration test, by counting the number of the migrated cells. The expression of the chemokine receptor 2 (CKR-2) in the induced and differentiated BMSCs was detected with the flow cytometry. Results The cells could be cultured with the methods of differential adhesion and density gradient centrifugation and still had higher prol iferative and differentiative potency; the induced cells at the 3rd passage could differenciate to the osteoblasts, confirming that the cells were BMSCs; the myogenic induced BMSCs possesed the sarcotubule structure. The number of the migrating BMSCs at MCP-1 concentrations of 25-400 ng/ mL were respectively 35.066 7 ± 6.584 2, 43.200 0 ± 6.460 8, 44.466 7 ± 4.823 5, 45.600 0 ± 8.650 3, and 50.733 3 ± 7.582 5; showing significant difference when compared with control group (28.333 3 ± 8.917 6, P lt; 0.05), and presenting significant difference among 25, 50, 400 ng/mL groups compared with each other (P lt; 0.05). The expression of CKR-2 in the mouse BMSCs (48.0%) was significantly higher (P lt; 0.001) than those of blank control (0.6%) and negative control (17.0%). Conclusion The results indicate that the MCP-1 can induce the migration of mouse BMSCs by MCP-1/CKR-2 pathway.

    Release date:2016-08-31 05:48 Export PDF Favorites Scan
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