正常人间围血及骨髓单个核白细胞和白血病肿瘤细胞的免疫分型

本文用10种单克隆抗体(McAb)分析了正常人周围血及有髓单个核细胞的免疫表型,以及急性淋巴细胞白血病(ALL)和急性髓细胞白血病(AML)的免疫表型,并以免疫双酶标记法观察了非T-ALL肿瘤细胞的肿瘤相关核仁抗原(HMNA)和细胞表面抗原的表达。结果:不同年龄正常群体周围血CD_4~+细胞数及CD_4/CD_8比值有差异;约3％的正常骨髓单个核细胞CD_(10)~+(ALL的抗原)。应用单克隆抗体对白血病的免疫分型,不仅能确诊肿瘤的谱系,还能了解细胞分化阶段。本文讨论了AML和ALL免疫分型中的鉴别性McAb。HMNA为多种肿瘤细胞的标记,本文观察到幼稚B细胞白血病及毛细胞白血病的肿瘤细胞中HMNA亦为阳性。     

THE HISTOCHEMICAL DEMONSTRATION OF GLYCERALDEHYDE-3-PHOSPHATE DEHYDROGENASE ACTIVITY

A histochemical method for demonstration of glyceraldehyde-3-phosphate dehydrogenation by tissues is described. The method utilizes Nitro BT as an indicator, glyceraldehyde-3-phosphate obtained from hydrolysis of commercially obtainable glyceraldehyde-3-phosphate diethylacetal (monobarium salt) as substrate, and (ethylenediamine)tetraacetic acid acid disodium as an activating agent in a medium buffered to pH 7.2 by 0.2 M sodium phosphate. The heat lability, substrate and coenzyme specificity, and sulfhydryl and phosphate dependence of the tissue component catalyzing this reaction indicate that glyceraldehyde-3-phosphate dehydrogenase activity is being demonstrated. The disparity between the known pH optimum of this enzyme and that determined histochemically, and the anomalous histochemical localization to mitochondria of this enzyme which has been found in the soluble fraction by differential centrifugation, are thought to result from the diaphorase dependence of the tetrazolium methods and to emphasize the need for caution in the interpretation of histochemically determined intracellular localization of dehydrogenating enzymes. The evidence gathered by previous workers concerning the feasibility of demonstrating specific dehydrogenases with Nitro BT, and the correspondence of the distribution of glyceraldehyde-3-phosphate dehydrogenase determined histochemically with available quantitative data, suggest that at the cellular level the histochemical results accurately reflect the distribution of this enzyme.     

THE PROLIFERATIVE STATE OF GRANULOCYTIC PROGENITOR CELLS IN HUMAN BLOOD AND MARROW

A double layer agar technique was used to investigate the proliferative state of granulocytic progenitor cells (Colony Forming Units in Culture; CFUc) in human peripheral blood and bone marrow. The sensitivity of the progenitor cells to the S-phase specific agent, hydroxyurea, was used as an index of the proportion of cells engaged in DNA synthesis. In the presence of low concentrations of colony stimulating factor (CSF) the CFUc were found to be virtually insensitive to the drug. However, when cultured in the presence of increasing concentrations of CSF the proportion of CFUc apparently killed by hydroxyurea increased to a maximum of 23% for those cells in the blood and 39% for those in the marrow. The results indicate that CFUc which are slowly proliferating are sensitive to low concentrations of CSF. In contrast, those CFUc which are proliferating more rapidly require high concentrations of CSF before they will form colonies in culture. A model has been devised which suggests that as CFUc mature, their cell cycle time shortens and their sensitivity to CSF decreases.     

体外培养骨髓巨核细胞脱氢酶活性的细胞化学观察

本文采用液体培养体系结合酶细胞化学方法,对体外培养不同发育阶段的小鼠肾髓巨核细胞乳酸脱氢酶、苹果酸脱氢酶、谷氨酸脱氢酶的活性变化进行了动态观察。在9天培养期间,巨核细胞的增殖数在5—7天达到高峰,并随时间有不同程度分化。对培养3、5、7、9天的巨核细胞进行酶细胞化学研究,结果表明,巨核细胞在发育成熟前,三种酶活性均有增高。提示巨核细胞在分化过程中,糖酵解及三羧酸循环代谢均有增强。     

β-半乳糖苷酶基因在正常人及白血病人骨髓细胞的表达

为探索组织化学方法检测标志基因在正常骨髓细胞及白血病细胞的表达,本研究利用脂质体介导将ＮｅｏＲ基因和ＬａｃＺ基因共转移正常人及白血病人骨髓细胞。然后,采用Ｘ－ｇａｌ染色的方法,我们观察了ＬａｃＺ基因在转导细胞的表达。结果显示：ＬａｃＺ基因在正常人及白血病人骨髓细胞表达的阳性率分别为１３．３３％±２．６８％和１５．３９±３．６９％。经Ｇ４１８筛选后,转导阳性细胞率达到４６．０６％±３．４７％和４８．２２％±４．４７％。提示：经脂质体介导ＬａｃＺ基因在正常骨髓细胞及白血病细胞可获得高效的转移率。同时表明,利用组织化学方法可有效地检测标志基因的表达。     

培养骨髓基质细胞的尿嘧啶核苷二磷酸半乳糖-4-表异构酶活性

本实验用液体静置法体外培养小鼠骨髓基质细胞。用细胞化学法观察处于不同分化阶段基质细胞中的尿嘧啶核苷二磷酸半乳糖－－４－表异构酶（Ｕｒｉｄｉｎｅｄｉｐｈｏｓｐｈｏｇａｌａｃｔｏｓｅ－４－ｅｐｉｍｅｒａｓｅ,ＵＤＰＧａｌ,ＥＣ５．１．３．ａ）活性。结果在各类骨髓基质细胞中均可见到很强的酶反应。在由原始网状细胞向成熟星状细胞分化过程中,酶活性逐渐增强。随着培养时间和延长（培养５、７、１０天）,星状细胞和成纤维细胞中酶反应的阳性率和阳性度逐渐增高。这证明在体外培养骨髓基质细胞中由ＵＤＰＧａｌ催化的代谢非常活跃     

THE PROLIFERATION OF LYMPHOID CELLS IN GUINEA-PIG BONE MARROW

A double isotope DNA labelling method has been used to determine the duration of DNA synthesis (S) in bone marrow lymphoid cells classified by their nuclear diameters in smears. Incorporation of ³H-thymidine was confined almost entirely to marrow lymphoid cells of 8·0-15·0 μm nuclear diameter (large lymphoid cells). After exposure to ³H-thymidine in vivo and ¹⁴C-thymidine 40-104 min later in vitro , the proportion of cells labelled with ³H alone to those labelled with ¹⁴C(±³H) in radioautographic smears, plotted against time indicated the efflux from S per hour. Collectively, 28·3 ± 1·1% of all large lymphoid cells were in S and the efflux from S was 15·1% per hour. With decreasing cell size (nuclear diameter) the efflux fell progressively from 28·3% per hour (11·0 μm) to 9·2% per hour (8·0-8·9 μm) and the proportion of cells in S declined from 54·9 ± 2·3% to 14·8 ± 1·6%. Influx into S, measured in vitro by reversing the sequence of isotopes, closely resembled the corresponding efflux values in vivo relative to cell size. Most DNA synthesizing marrow large lymphoid cells belonged to a subgroup with deeply basophilic cytoplasm. The results demonstrate that basophilic large lymphoid cells in the marrow are actively proliferating and have a mean S phase duration of 6·6 hr. The largest marrow lymphoid cells (11·0 μm) proliferate most rapidly (S phase, 3·5 hr; maximum cell cycle time, 6·4 hr) while S duration is prolonged progressively to 10·9 hr for the smaller cells (8·0-8·9 μm).     

正常小鼠骨髓血红蛋白含量的测定

小鼠骨髓血红蛋白含量的变化可以间接地反映骨髓微循环系统形态和功能的状况。按Burger and Knyszynski(1969)方法操作繁复,限制了它的推广应用及正常值的问世。最近,我们建立的简易测定方法,为成批标本的测定和正常值的确定创造了条件。 正常小鼠骨髓血红蛋白含量测定的目的:1)在较大量标本的测定中进一步验证该方法的可靠性;2)确定青、成年小鼠骨髓血红蛋白的正常值范围;3)分析其可能的影响因素,以便更好地控制实验条件和判断骨髓微循环障碍的程度。     

THE NUMBER AND POSSIBLE FUNCTIONS OF DNA-SYNTHESIZING CELLS IN HUMAN BLOOD

The number of DNA-synthesizing cells in the blood of patients with various disorders was studied autoradiographically after incubation of blood in vitro with [³H]thymidine. The DNA-synthesizing cells were cytologically assigned to the following categories: erythroid, myeloid, lymphoplasmacytoid and unidentifiable (monocytoid or blast-like) cells. The following patient categories were studied: mitral valvular disease (samples obtained from peripheral vein, pulmonary artery and left auricle), ‘autoimmune diseases’(systemic lupus erythematosus, schleroderma, Hashimoto's thyroiditis, immunohaemolytic anaemia), patients with depressed haemopoiesis (aplastic anaemia, nitrogen-mustard induced bone-marrow hypoplasia) and with increased haemopoiesis (haemolytic anaemia, pernicious anaemia before and during initial vitamin-B₁₂ therapy, red-cell mass regeneration after haemorrhage or iron deficiency) and patients with bacterial infection. In all conditions studied, the number of labelled monocytoid and blast-like cells varied between 0 and 4/μl. Similarly, the number of labelled lympho-plasmo-cytoid cells was consistently low (0–8/μl) in all cases studied except two, where values of 37 and 63/μl were found. Both these patients had severe bacterial infections. The function(s) and potential(s) of these cells are discussed. The fate of the blast-like and monocytoid cells remains obscure. The lympho-plasmocytoid cells probably serve an immunological function, perhaps by disseminating immune responses. Whether or not some DNA-synthesizing cells in the blood are haemopoietic stem cells cannot be decided from the available evidence.     

人胎儿呼吸道肥大细胞的组化特征及其共与其它细胞的关系

用组织化学技术方法 ,我们对 5 0例不同胎龄人胎儿的鼻粘膜和气管的组织内的肥大细胞组织化学特征以及其与周围其它细胞的关系进行了研究。结果发现 :随着胎龄的增加 ,肥大细胞的颗粒甲苯胺蓝 (TB)染色时从浅紫色加深至深紫色 ,Alcian蓝·藏红 (AB· S)染色呈从蓝色到出现红色、红蓝混合染色的变化 ,临界电解质浓度 (CEC)值和硫酸小蘖碱荧光染色强度逐渐增高 ;多见肥大细胞与成纤维细胞、淋巴细胞和毛细血管内皮等密切接触 ,且出现在神经内、外膜之中。这提示 :1肥大细胞的发育成熟与胎儿呼吸道器官的发育是相关的。 2肥大细胞可能参与细胞、组织的分化成熟。     

THE DEVELOPMENT OF FIBROBLAST COLONIES IN MONOLAYER CULTURES OF GUINEA-PIG BONE MARROW AND SPLEEN CELLS

In monolayer cultures of guinea-pig bone marrow and spleen the development of discrete fibroblast colonies takes place on days 9–12. The linear increase in the number of colonies with increasing numbers of explanted cells and the distribution of male and female cells in mixed cultures support the view that fibroblast colonies are clones. The concentration of colony-forming cells in bone marrow and spleen is approximately 10^-5. Bone marrow culture (but not spleen culture) fibroblasts are capable of spontaneous bone formation in diffusion chambers. Fibroblasts from both bone marrow and spleen cultures are inducible to osteogenesis in diffusion chambers in the presence of transitional epithelium.     

GROWTH OF MOUSE AND HUMAN BONE MARROW IN DIFFUSION CHAMBERS IN MICE

Both murine and human bone marrow cells were cultured in plasma clots which were formed inside diffusion chambers implanted into cyclophosphamide- and saline-treated mice. After an initial fall, the number of mouse bone marrow cells and numbers of mouse myeloid stem cells (CFU-C) and agar cluster-forming units rose faster in the cyclophosphamide-treated animals. These hosts also favored formation of myeloid (CFU-D-G) and erythroid (CFU-D-E) colonies and myeloid clusters in the plasma clot. The number and growth rate of mouse CFU-D-G were higher than those of CFU-C from the same marrow population. These observations suggest the existence of humoral factors stimulating granulocyte progenitor cell replication and differentiation. At its best the increment of CFU-D-E number was equivalent to that caused by a single 0·1 unit erythropoietin dose. Culture of normal human marrow cells resulted in colonies in the plasma clot containing only granulocytes and macrophages. Cyclophosphamide-treated host animals were essential for human CFU-D-G development. Plating efficiency for human marrow myeloid colonies was better in the conventional in vitro agar cultures than in diffusion chambers.     

骨髓基质细胞与交联明胶-聚羟基丁酸酯膜的生物相容性研究

目的研究生物材料交联明胶-聚羟基丁酸酯膜与骨髓基质细胞的生物相容性,探讨新型材料在骨组织工程中的应用前景。方法体外培养兔骨髓基质细胞,分别接种于G-PHB(交联明胶-聚羟基丁酸酯)、PHB(聚羟基丁酸酯)和G(交联明胶)材料膜片。采用MTT法检测细胞增殖活性,体视学方法检测细胞粘附能力,荧光双染法检测细胞完整性,扫描电镜观察细胞-材料界面。结果MTT检测发现G-PHB组增殖活性最强,而且表现为最佳的细胞粘附特性,与对照组比较差异有显著性意义。各组细胞完整性分析没有发现显著性差异。扫描电镜观察显示,G-PHB组细胞粘附及铺展良好,优于其他各组。结论交联后的生物降解膜材料G-PHB与BMSCs细胞的体外相容性明显优于单纯膜材料PHB和明胶,在骨组织工程学领域具有良好的研究价值和应用潜力。     

A HISTOCHEMICAL ENZYME KINETIC SYSTEM APPLIED TO THE TRYPSIN-LIKE AMIDASE AND ESTERASE ACTIVITY IN HUMAN MAST CELLS

A method for the determination of enzyme kinetic constants V_m, K_m, and K_i in a histochemical system has been devised. As a substitute for the reciprocal of the reaction velocity, the times necessary to reach a fixed amount of end product (the initial visible color) in a tissue site at various substrate concentrations are plotted, according to the method of Lineweaver and Burk, against the reciprocal of the substrate concentrations. The technique as applied to trypsin-like esterase and amidase activities in human mast cells indicates that a single enzyme or closely related enzymes in this site are responsible for the hydrolysis of both the amide and ester substrates and that typical trypsin substrates act as competitive inhibitors of their hydrolysis. Parallel biochemical studies were performed to evaluate the effect of certain aspects of the experimental histochemical method on a purified homospecific enzyme. The relative kinetic constants derived by the histochemical method afford a further means of characterizing enzymic activity in a histochemical system.     

人血树突状细胞培养后的形态及抗肿瘤活性

观察新鲜分离和经体外培养３６小时的人外周血树突状细胞ＤＣ。和ＤＣ３６的形态学及其对淋巴因子与植物血凝素激活的杀伤细胞（ＬＰＡＫ细胞）体外诱导人肝癌细胞株ＢＥＬ┐７４０２的促进作用。形成学观察用免疫细胞化学法。抗肿瘤实验分为三大组：（１）Ｌ组（ＢＥＬ┐７４０２＋ＬＰＡＫ）,（２）ＬＤ３６组（ＢＥＬ┐７４０２＋ＬＰＡＫ＋ＤＣ３６）,（３）ＬＤ０组（ＢＥＬ┐７４０２＋ＬＰＡＫ＋ＤＣ０）。各组均采用ＬＰＡＫ与ＢＥＬ┐７４０２为５∶１和１０∶１两种效靶比。培养４８小时后用中性红摄入比色法检测ＬＰＡＫ细胞的杀伤活性。结果显示,ＤＣ３６的形态以具有细长突起者为多,与ＤＣ０主要为园形或具有短而钝突起的形态有明显差别。各组的细胞毒活性依次为：ＬＤ３６组＞ＬＤ０组＞Ｌ组（Ｐ＜０．０１）,并随效靶比增高而相应增强。这表明新鲜分离的人外周血ＤＣ在体外经３６ｈ培养后,不仅在形态上成熟,而且抗肿瘤活性也明显增强     

骨髓基质干细胞诱导分化为神经元过程中miR-124和miR-128的表达

目的探讨骨髓基质干细胞诱导分化为神经元过程中miR-124和miR-128的表达变化及作用。方法采用全骨髓培养法体外分离培养获得骨髓基质干细胞,取传代培养至第3代的骨髓基质干细胞,在神经干细胞培养液及细胞因子等条件下诱导其分化为神经元,倒置显微镜下观察其形态变化,应用ABI公司的TaqManMicroRNAAssaysreal-timePCR技术,检测miR-124和miR-128在诱导分化过程中的表达。结果 miR-124分化后神经元的表达是未分化BMSCs的0.051倍(P0.05);miR-128分化后神经元的表达是未分化BMSCs的0.070倍(P0.05)。结论 miR-124和miR-128在骨髓基质干细胞诱导分化为神经元过程中可能起重要作用。     

人骨髓细胞培养液中干细胞刺激物的分析研究

人骨髓细胞体外培养液中含有高活力的 CSF,在长期培养过程中,CSF 活力的变化,与 CFU-C 数量的变化有大致平行的趋势。这种 CSF 对狗和小鼠也同样有效。人骨體条件液中的 CSF 对培养中的 CFU-S 也有明显的激发作用。这一结论可以从几个方面获得证据:第一,小鼠骨髓细胞与人骨髓条件液保温六小时后,再测定其中 CFU-S 数,结果是增加了。第二,经亚致死剂量照射的小鼠,腹腔注射适量的人骨髓条件液,其内源性脾结节也明显增多。第三,采用阿糖胞苷自杀的方法,测定小鼠骨髓经与人骨髓条件液保温后,其中 CFU-S 的自杀率也有增高的趋势。上述几方面的实验,说明人骨髓长期培养中存在着某种活性物质,调节体外造血。至于这种物质的来源,以及在体外造血中所起的作用,还需要做很多工作,逐步予以澄清。