恶性肿瘤患儿自体外周血CD_(34)^+造血干细胞的动员和检测

目的探讨恶性肿瘤患儿经化疗和细胞因子动员后，外周血CD造血干细胞的含量变化及意义。方法恶性肿瘤患儿6例，经化疗和细胞因子动员后，用CD抗体标记，流式细胞仪检测外周血CD细胞18次，对测定结果进行统计学分析。结果6例患儿的CD细胞的百分率为1．78％～9．72％，较正常儿童外周血的含量增加17～97倍，CFU-GM增加19～74倍。三组不同疾病：NHL、ANLL和ALL之间CD细胞含量有显著性差异，P＜0．01。结论恶性肿瘤患儿经动员后，CD造血干细胞及CFU-GM有明显扩增，CD的检测在自体造血干细胞移植中具有重要的意义。

以逆转病毒介导对人脐血CD_(34)^+造血细胞进行人MDR1基因转染的实验研究

探讨逆转录病毒介导的MDR1基因转导入脐血CD34+细胞的最佳方法,为MDR1基因转导的临床应用打基础。方法:用磷酸钙沉淀法将含有人全长MDR1cDNA的逆转录病毒载体pHaMDR1/A转到包装细胞PA317中,建立产病毒细胞系,以人脐血中分离的CD34+造血干/祖细胞为靶细胞,在体外进行基因转染,转导的条件为:与含病毒的上清液共培养12天,每天更换病毒上清液,上清液中加入IL-3,IL-6和SCF三种造血生长因子(HGF),转染后用集落培养法测定对COL的耐药性,用PCR检测14～17天所形成集落的MDR1cDNA,计算转染率,用免疫组化法检测P170的阳性程度,并观察不同时间间隔加HGF对脐血CD34+细胞的扩增和转染的影响。结果:脐血CD34+细胞转染阳性为86.4%,P170的阳性率为77.0%,77.1%的集落对6ng/ml的COL耐受,57.4%的集落对7ng/ml的COL耐受。结论:此转染系统既能有较好的转导效果,也有较好的扩增效果,有一定的临床实用价值。

脐血CD_(34)^+细胞免疫表型的分析

应用免疫磁珠法分离脐血CD细胞，以比较CD细胞亚群及各系相关抗原的变化。经过分离，CD细胞由1．47±0．77％升至57．39±16．17％，分离后CDCD细胞占CD细胞的比率为7．82±4．79％CD。细胞纯化同时可减少CD细胞达14．12±9．18倍，CD细胞减少16．42±21．47倍；B系（CD(19)）、巨核系（CD(41)）、NK系（CD(56)）各抗原表达率在CD细胞分离后均明显降低。结论：CD细胞纯化可明显减少CD细胞，应用纯化的CD细胞进行移植应加强支持治疗。

rhTPO对CD_(34)^+细胞增殖及形成CFU-MK作用的研究

目的研究重组人TPO（rhTPO）单独及与rhIL-3、rhIL－6、rhSCF协同体外对巨核系的增殖效应。方法采用纯化的CD+34细胞，进行求固体巨核细胞集落培养和液体悬浮培养，研究TPO及与IL－3、IL－6、SCF协同体外对CD+34细胞增殖及向巨核系空向分化的特性，和形成CFU－MK的作用。结果rhTPO可以诱导CD+34细胞形成CFU－MK，增加巨核细胞集落数，这种作用可以被rhIL－3、rhIL－6、rhSCF增强。液体培养中，rhTPO促进CD+34变细胞分化／成熟为表达GPⅡb／Ⅱa的细胞，增加体系中CD+34。细胞，rhIL-3、rhIL－6、rhSCF可以协同TPO的作用。结论TPO作为一种促增殖因子，促进巨核系祖细胞的增殖及分化。

低温冷冻对脐血CD_(34)^+细胞和造血祖细胞增殖的影响

采用－８０℃低温冷冻法，观察冷冻前及冷冻后１、２、３周时单个核细胞（ＭＮＣ）的回收率，脐血造血前体细胞在体外的增殖力，并用流式细胞仪检测ＣＤ３４＋细胞的百分率。旨在探讨低温冷冻对脐血造血前体细胞的影响。结果表明：脐血冷冻后１、２、３周时ＭＮＣ的回收率分别为９３．６％，９１．５％和９０．７％（Ｐ＞０．０５）；细胞活力分别为９８％，９７％，９５％和９１％（Ｐ＞０．０５）；ＣＤ３４＋细胞依次为１．２０％、１．１８％、１．１６％和１．１７％；ＣＦＵ－ＧＭ，ＣＦＵ－Ｅ冷冻后１、２周时回收率达９７％和９５％（Ｐ＞０．０５），第３周时达８９％（Ｐ＞０．０５）。结果提示：长期冷冻可能导致冷冻之脐血祖细胞产率下降，但对代表造血干细胞的ＣＤ３４＋细胞影响则不大。

IL-15对MDS CD_(34)^+细胞的诱导分化作用探讨

目的 观察IL - 1 5对体外培养的MDSCD3 4+ 细胞的诱导分化作用 ,方法 应用MACS免疫磁珠分离系统提取高纯度MDS骨髓CD3 4+ 细胞 ,建立以造血生长因子为基础的体外培养体系 ,用不同浓度的IL - 1 5作用CD3 4+ 细胞 ,流式细胞术检测培养后的细胞单克隆抗体分化和细胞周期的表达 ,细胞化学染色观察细胞形态变化。结果 应用MACS方法成功提取MDSCD3 4+ 细胞 ,体外培养MDSCD3 4+ 细胞生长情况一般 ,IL - 1 5作用后MDSCD3 4+ 细胞出现明显分化 ,细胞形态学显示细胞向成熟转化 ,实验组的单抗表达水平CD71、CD3 3 、CD19、CD13 均较对照组为高 ,细胞周期分化。结论 IL - 1 5对MDSCD3 4+ 细胞有一定的诱导分化作用 ,IL - 1 5对MDS可能有一定的治疗应用前景。

羟基淀粉沉淀对免疫磁珠法分离脐血CD_(34)^+细胞及造血祖细胞增殖功能的影响

目的 :应用羟基淀粉沉淀去除脐血红细胞和免疫磁珠 (MACS)阳性选择 ,建立富集、分离脐血CD34+ 细胞的简易实用方法 ,通过造血祖细胞集落培养分析其在细胞因子作用下的增殖潜能 ,观察羟基淀粉沉淀对造血细胞增殖功能的影响。方法 :采用羟基淀粉沉淀和改进的 MACS富集、分离脐血 CD34+细胞 ,以甲纤半固体造血细胞培养法观察其粒 -单系细胞 (CFU- GM)和红系爆式集落 (BFU- E)的数量和特性。结果 :脐血分离前 ,CD34+细胞纯度为 1.5 %～ 3% ,MACS分离后其纯度可达 85 % ,羟基淀粉沉淀和 MACS分离可达 91% ;CD34+造血祖细胞培养有明显的增殖 ,采用 IL - 3、IL - 6、SCF、GM- CSF、EPO等细胞因子组合扩增培养 9～ 14d,CD34+ 细胞在液体培养中有明显扩增 ,MACS分离后 CD34+ 细胞总数增加 39倍 ,羟基淀粉沉淀和 MACS分离可增加 45倍。结论 :应用羟基淀粉沉淀和改进的 MACS系统可有效富集、分离脐血 CD34+细胞 ,羟基淀粉沉淀对 CD34+细胞的富集、分离无影响 ;脐血细胞分离后作造血祖细胞培养 ,可产生丰富的 CFU- GM和 BFU- E,说明羟基淀粉沉淀分离的 CD34+ 细胞的增殖功能优于 MACS分离 CD34+ 细胞的增殖功能。

高血压脑出血后外周血CD_(34)^+、CD_(166)^+与白细胞水平的动态变化及意义

为了解高血压脑出血患者血中干细胞变化情况,动态监测脑出血后外周血CD_(34)^+、CD_(166)^+细胞的绝对值和白细胞的动态变化,采用流式细胞仪和全自动细胞分析仪对高血压脑出血患者40例,分轻症组(血量11～30 ml)和重症组(血量31～50 ml)各20例,取同年龄段20例健康患者作为对照组。分别于第3、7、14、30天各采外周血2ml,肝素抗凝,进行动态监测CD_(34)^+、CD_(166)^+细胞的绝对值和白细胞的变化。结果表明,高血压脑出血后外周血CD_(34)^+、CD_(166)^+细胞和白细胞的绝对值均不同程度地上升,轻症组和重症组CD_(34)^+、CD_(166)^+细胞数分别于第7、14天达高峰,之后逐渐下降,重症组上升幅度较大,与对照组比较第7天具有明显统计学意义(P<0.05);与轻症组比较第14天具有明显差别(P<0.05)。两组白细胞数上升迅速,恢复也较快。轻症组和重症组分别于第7天和14天恢复至正常范围;待CD_(34)^+、CD_(166)^+细胞数达高峰时,白细胞已恢复至正常,与CD_(34)^+、CD_(166)^+细胞变化呈负相关(r=-0.284,P=0.041;r=-0.458,P=0.043)。结论显示高血压脑出血后CD_(34)^+、CD_(166)^+细胞及白细胞不同程度地上升,且重症患者上升幅度较大,表明这可以作为高血压脑出血后自身修复潜能及病情轻重的重要观察指标,同时脑出血后机体存在CD_(34)^+、CD_(166)^+细胞动员,亦表明脑出血后机体存在内源性干细胞的动员,参与脑出血后神经功能的修复。

心理干预对老年难治性急性早幼粒细胞白血病骨髓CD_(34)^+细胞bcl-2表达的影响

目的探讨心理干预治疗难治性急性早幼粒细胞白血病(acute promyelocytic leukemia,APL)的临床疗效及作用机理。方法将71例难治性APL老年患者随机分为治疗组(36例)和对照组(35例),对照组采用复方青黛片常规治疗,治疗组在常规治疗基础上加用心理干预治疗。观察临床疗效及不良反应,并分别于治疗前后采用单克隆抗体-免疫磁珠分离系统(MACS)分离、纯化骨髓CD_(34)^+细胞;用SABC亲和细胞法和CMIAS系列多功能真彩图像分析仪检测骨髓CD_(34)^+细胞bcl-2表达。结果治疗组和对照组的完全缓解率、部分缓解率、总有效率分别为86.11%,8.33%,94.44%和74.29%,2.85%,77.14%.治疗组疗效明显优于对照组(P<0.01)。两组骨髓CD_(34)^+细胞bcl-2蛋白阳性产物的阳性率和OD值治疗前均较健康组明显增高(P<0.01),治疗后显著减低(P<0.01),治疗组减低幅度尤为明显,与对照组比较差异有显著性(P<0.01)。结论耐心细致的心理护理可明显提高中药砷剂的临床疗效和安全性;其作用机制可能是通过心理干预配合中药砷剂治疗能更有效下调凋亡抑制基因bcl-2表达,诱导或促进了APL骨髓CD_(34)^+细胞的分化和凋亡,使骨髓正常造血功能得以恢复重建。

脑外伤病人外周血CD_(34)^+细胞及白细胞含量的动态变化

为动态观察并探讨不同损伤程度的颅脑损伤病人外周血白细胞及CD_(34)^+细胞的变化及同预后的关系,以及二者升高的机制和临床意义,选取我院神经外科收治的伤后6h内入院脑外伤病人,按入院时格拉斯哥昏迷评分(Glasgow coma sale,GCS)分为轻重两组,同时选择我院体检中心健康成年人15名,作为对照组。于入院第1天、第3天、第5天、第7天、第11天、第14天抽取静脉血,用流式细胞仪检测外周血CD_(34)^+细胞含量;用血细胞分析仪常规检测白细胞计数,同时观察病情变化,追踪预后,按照病人预后不同情况分成死亡组和生存组,比较分析相关数据。结果表明,30例颅脑损伤病人外周血白细胞及CD_(34)_^+细胞数量随病程的发展均有不同程度的升高,损伤越重、GCS评分越低,白细胞及CD_(34)^+细胞计数越高,预后越差,白细胞升高持续时间越长,预后愈差。外周血CD_(34)^+细胞在颅脑损伤后轻、重两组病人,各时间段逐步升高。重症病人自第3天与正常对照组出现统计学差异,明显高于轻症组病人,轻、重症两组间比较,在第7、11、14天有统计学差异。白细胞计数在伤后迅速升高并逐步下降,同CD_(34)^+细胞变化未见正相关。本研究认为,外周血白细胞及CD_(34)^+细胞,在颅脑损伤病人急性期均有不同程度的升高,计数增高越明显,持续时间越长,结果预后越差。外周血白细胞及CD_(34)^+细胞计数的变化可以成为判断其预后的重要指标。

Expression of Caspase－3 in Cord Blood CD34^＋ Cells during Culture in vitro

Objective: To investigate the expression and significance of caspase-3 protein in CD34^+ cells from cord blood (CB) during culture in vitro with different growth factors. Methods: RT-PCR, Western blot and flow cytometry techniques were used to detect the expression of caspase-3 in CD34^+ CB cells during culture in vitro. Results: Caspase-3 mRNA was constitutively expressed at a low level in freshly isolated CD34^+ cells. The expression of caspase-3 mRNA and protein was upregulated when these cellswere first expanded in suspension culture with growth factors for 3 days. However, only the 32 kDa inactive caspase-3 proenzyme was detected in the freshly isolated CD34^+ cells as well as during the first 3 days expansion with cytokines. With longer culture time in vitro, especially in the presence of the combination of IL-3, IL-6 and GM-CSF, caspase-3 was activated and a cleavage product of 20 kDa became detectable.Conclusion: Caspase-3 is involved in apoptosis of primitive CB CD34^+ cells during expansion in vitro.

Effect of Homoharringtonine on Bone Morrow CD34^+CD7^+ Cells in Chronic Granulocytic Leukemia

Objective： To explore the effect of homoharringtonine （HHT） on bone morrow CD34^＋CD7^＋ cells in chronic granulocytic leukemia （CGL）. Methods： The changes of bone morrow CD34^＋CD7^＋ cells were observed after the treatment of HHT in 23 cases with CGL. The proliferation and apoptosis of CD34^＋CD7^＋ cells treated with HHT in vitro were studied. Results： The proportion of CD34^＋CD7^＋ cells in CGL （0.145±0.021） was higher than that of normal control （0.052±0.013）. The proportion of CD34^＋CD7^＋ cells in patients who got cytogenetic responses to HHT （0.072±0.020） decreased remarkably, but not in those patients who did not got cytogenetic responses to HHT, （0.137±0.023）. the proliferation of CD34^＋ cells was inhibited and the proportion of CD34^＋CD7^＋ cells decreased after cultured with HHT （0.134 in 24 h, 0.126 in 48 h and 0.102 in 72）. The apoptosis rate of CD34^＋CD7^＋ cells was higher than that in CD34^＋CDT cells （35.39%±4.39% versus 24.57%±4.01%, P〈0.05） 72 h after culture with HHT. Conclusion： The proportion of CD34^＋CD7^＋ cells in CGL was higher than that of normal control and HHT may inhibit the proliferation and induce apoptosis of bone marrow CD34^＋CD7^＋ cells.

PERIPHERAL BLOOD CD34^+ CELL MOBILIZATION IN 42 PATIENTS WITH SEVERE AUTOIMMUNE DISEASE

Objective To evaluate the feasibility and safety of peripheral CD34+ cell mobilization in patients with severe autoimmune disease. Methods Forty-two patients underwent a total of 46 mobilizations by the regimen of cyclophosphamide 2-3 g/m2 +recombinant human granulocyte colony stimulating factor (rhG-CSF) 5 μg·kg-1·d-1. The positive selection of CD34+ cell was performed through the CliniMACS. Results In 8.1±2.3 days after administration of cyclophosphamide, the peripheral white blood cell and mononuclear cell (MNC) decreased to the lowest level. In 3.7±1.6 days after injection of rhG-CSF, the peripheral absolute MNC and CD34+ cell counts were 0.95×109/L and 0.035×109/L, respectively. After 2.4±0.6 times of leukapheresis, there gained 4.46×108/kg of MNC and 5.26×106/kg of CD34+, respectively. After mobilization, the underlying diseases were ameliorated more or less. In systemic lupus erythematosus (SLE) patients, SLE Disease Activity Index (SLEDAI) decreased from a median of 17 to 3 (P<0.01). In rheumatic arthritis patients, an American College of Rheumatology criteria for 20%(ACR20) response was achieved in all five patients. Totally, 17.4% of patients whose absolute neutrophil count <0.5×109/L suffered infection, and 31.0% of patients had bone pain after the injection of rhG-CSF. Two patients suffered severe complications, one with acute renal failure and recovered by hemodialysis, the other died of thrombotic thrombocytopenic purpura. Failed mobilization occurred in three patients. Conclusions Sufficient CD34+ cells can be mobilized by low dose of cyclophosphamide and rhG-CSF. CD34+ cell mobilization for treatment of severe autoimmune disease not only is appropriate in both effectiveness and safety but ameliorates disease also.

Exploring hematopoietic stem cell population in human milk and its benefits for infants:A scoping review

Objective:To comprehensively explore hematopoietic stem cells(HSCs)in human milk,understanding their molecular markers,isolation methods,benefits for infants,and potential medical applications.Methods:We conducted a scoping literature review following the PRISMA-ScR guidelines.This review included studies investigating HSCs in human milk,utilizing molecular markers such as CD34^(+),CD113^(+),and CD117^(+)for characterization.Both in vitro and in vivo studies exploring the morphology,function,and clinical implications of these cells were considered.The diverse range of papers reviewed were indexed in PubMed,Science Direct,Scopus,Sage Journals,and Google Scholar,published between 2010 and 2023.Results:This scoping review explored 577 articles and selected 13 studies based on our inclusion criteria,focusing on HSCs in human milk.Most studies dilute samples prior to HSC isolation,followed by detection using markers such as CD34^(+),CD113^(+),and CD117^(+),with flow cytometry serving as the primary analysis tool,focusing on their isolation and detection methods.While no definitive benefits have been conclusively established,there is a strong belief in the potential of HSCs to positively impact infant immunity,growth,and tissue repair.Conclusions:This review presents significant evidence supporting the presence of HSCs in human milk,identified by markers such as CD34^(+),CD113^(+),and CD117^(+).These cells show considerable potential in enhancing infant health,including immunity,tissue repair,cognitive development,and gastrointestinal health.Despite methodological variations in isolation and detection techniques,the collective findings underscore the potential clinical relevance of HSCs in human milk.Moreover,this review highlights the noninvasive accessibility of human milk as a source of HSCs and emphasizes the need for further research to unlock their therapeutic potential.

Characteristics of Ex Vivo Expansion of Endothelial Progenitor Cells

Summary： The characteristics for the ex vivo expansion of the endothelial progenitor cells （EPCs） were explored, CD34^＋ cells were selected from umbilical cord blood mononuclear cells （MNC） by MiniMACS system, expanded under the same conditions as those for total MNC, coincubation of CD34^＋ and CD34 from the same donor for EPCs. In addition, the effects of vessel endothelial growth factor （VEGF） and passage on cell differentiation, expansion kinetics and apoptosis were examined, EPCs were determined and quantified by immunocytochemistry and flow cytometry, The results showed that both coculture of CD346＋ and CD34^- and total MNC led to a significant increase in the expansion of CD34^＋ cells as compared with CD34 enrichment （P〈0.05）. There was a tendency toward decreased apoptosis in cultures when early passage was performed immediately after cord like structures appeared. VEGF had no significant effect on apoptosis （P〉0.05）, These differentiated EPCs were positive for CD34^＋, von Willebrand factor （vWF）, KDR, CD31 staining and phagocytized acetylated low-density lipoprotein （LDL）. CD34^＋ cells accounted for （68.2±6,3） % of attaching （AT） cells at day 7 of culture. It was suggested the most efficient method to ex vivo expansion of EPCs was coculture of CD34^＋ and CD34^- or total MNC. Early passage makes cell apoptosis rate decrease. VEGF had no significant effect on ex vivo expansion of EPCs.

人脐血间充质干细胞对脐血CD_(34)^+细胞体外扩增作用的研究

目的探讨含人脐血来源的间充质干细胞(MSCs)体系在体外对脐血造血干细胞(HSCs)扩增作用。方法(1)用含人脐血MSCs及不同造血生长因子(HGFs)组合的无血清扩增体系对人脐血CD+34细胞进行体外扩增。(2)于扩增前及扩增后第6、12天分别用双色流式细胞仪动态检测HSCs表面抗原标记:CD+34、CD+34CD-38、CD+34CD+3、CD+34CD+19、CD+34CD+33和CD+34CD+41a细胞的含量。(3)按本实验室方法行体外半固体培养,观察扩增前后脐血细胞粒单核细胞集落形成单位(CFUGM)、爆式红系集落形成单位(BFUE)、混合集落形成单位(CFUMix)及高增殖集落形成单位(CFUHPP)集落形成情况。结果(1)含人脐血MSCs体系对脐血CD+34CD38细胞的扩增倍数在第6天和第12天分别为159和437倍。该亚群百分比在单纯因子组扩增第12天时为1.98%,而在含脐血MSCs组为9.98%,明显高于扩增前。(2)集落培养表明,含脐血MSCs组扩增第12天与扩增第6天相比,其CFUMix和CFUHPP的扩增倍数增加,而单纯因子组这两种集落的扩增倍数下降。(3)随扩增天数的增加,两组扩增体系中CD+34CD+3和CD+34CD+41a细胞均明显增加,而CD+34CD+19和CD+34CD+3细胞均明显减少。两组相比,含脐血MSCs组差异更显著。结论(1)含脐血MSCs体系不仅能扩增更原始的造血干/祖细胞(HSPC),且具有在短期内(12d)保持HSCs不耗竭。(2)含脐血MSCs体系对脐血CD+34细胞向定向祖细胞的扩增,主要为髓系及巨核系祖细胞,而对其向淋巴系祖细胞的扩增具有抑制作用。

骨髓增生异常综合征和再生障碍性贫血患者骨髓CD_(34)^+细胞测定

目的检测骨髓增生异常综合征(MDS)和再生障碍性贫血(AA)患者骨髓CD_(34)^+细胞占单个核细胞(MNC)的比率,以探讨二者可能的发病机制。方法用流式细胞术(FCM)检测22例MDS患者、13例AA患者及12例非血液病患者骨髓CD_(34)^+细胞占MNC的比率。结果AA组与对照组、AA组与MDS-RA组、AA组与MDS-RAEB组、MDS-RA组与MDS-RAEB组的骨髓MNC中CD_(34)^+细胞的比率的比较差异有统计学意义(P<0.05)。大多数重型AA(SAA)患者(3/4)及很少慢性AA(CAA)患者(1/9)的骨髓MNC中的CD_(34)^+细胞的比率<0.1%。结论骨髓CD_(34)^+细胞的检测有助于判断AA患者病情及MDS患者的预后,亦可用于鉴别AA和MDS。

Effect of intracranial transplantation of CD34^+ cells derived from human umbilical cord blood in rats with cerebral ischemia

As a source of transplantable stem cells, the CD34^＋ subpopulation in human umbilical cord blood （HUCB） has been used extensively to treat some hematopoietic system diseases. However, whether CD34^＋ cells hold the therapeutic potential to cerebral ischemia is unknown. The purpose of this study was to observe the recovery of neural function after transplantation of CD34^＋ cells derived from HUCB into ischemic cerebral tissue in rats.

Retroviral transduction of a mutant erbB-2 gene into human CD34^+ derived dendritic cells

Objective To successfully transduce a mutant erbB 2 gene into normal human CD34 + derived dendritic cells (DCs) and verify gene expression in these transduced dendritic cells Methods The packaging cell line PA317 was transfected with mutant erbB 2 gene DNA and the virus produced was used to infect packaging cell line PG13 The virus produced by PG13 was used to infect CD34 + derived dendritic cells by the spinoculation method using flasks coated with fibronectin material to facilitate retrovirus gene transter efficiency and the mutant erbB 2 gene expression was assessed by ABC staining and FACScan methods Results A mutant erbB 2 gene packaging cell line was produced and this mutant gene was transduced into human CD34 + derived DCs It was verified that the relatively large numbers of the transduced DCs expressed the mutant erbB 2 protein which was eradicated of the ability to transform mouse NIH3T3 fibroblast cells Conclusions Human DCs can be gene modified and these gene modified DCs may be useful in stimulating T lymphocytes for immunotherapy

聚乙二醇重组人粒细胞集落刺激因子对大鼠心肌梗死的影响

目的:研究聚乙二醇重组人粒细胞集落刺激因子(PEG-rhG-CSF,商品名津优力)对大鼠实验性心肌梗死的影响。方法:应用冠状动脉结扎心肌梗死模型,通过心肌梗死面积的定量组织学测定、心肌酶学检查、心肌小血管密度及心肌免疫组化染色等观测指标,评价给予津化力24h和2周后的治疗作用。结果:津优力给药1次及给药2周后,心肌梗死范围减小,心肌CK和LDH降低,心肌梗死治疗2周后,在心肌梗死区及交界区有CD_(34)^+细胞的存在,心肌小血管的密度增加。结论:津优力对大鼠心肌梗死模型有明确的治疗作用。