THE EFFECT OF NITROGEN MUSTARD ON THE HAEMOPOIETIC STEM CELLS OF THE BONE MARROW IN THE RAT

The sensitivity of haemopoietic stem cells to the action of nitrogen mustard has been investigated by transfusion of bone marrow from treated donor rats to recipients whose own haemopoiesis had been reduced to low levels by whole body X-irradiation. By measurement of the resultant erythropoiesis in the recipients with radioactive iron, a comparison of the repopulating ability of nitrogen mustard treated bone marrow with that of normal bone marrow could be made. It was found that although a dose of 0.9 mg/kg body weight reduces bone marrow cellularity to less than 10% of normal, repopulating ability is not decreased to much less than half the normal level. This is in contrast to the effects of X-radiation, which has a more marked effect on the stem cell population than on the differentiated marrow cells. Possible reasons for this difference are discussed. It could be that the proliferative or metabolic state of the cell plays a role, or that some repair mechanism is operative in the stem cells which does not exist in the differentiated cells.     

Akt基因转染对骨髓间充质干细胞缺氧时凋亡和增殖的影响

目的采用Akt基因转染鼠骨髓MSCs探讨Akt基因是否减轻MSCs缺氧时的凋亡和提高缺氧时的增殖能力,即耐缺氧能力。方法将转染和未转染Akt基因的MSCs置于94%N2、1%O2和5%CO2缺氧箱中37℃孵育不同时间（常氧、缺氧0.5h、1h、2h、4h和8h）后,Annexin V/PI双染法行流式细胞仪分析凋亡率（apoptoticrate,AR）和死亡率（deadrate,DR）、MTT法分析细胞增殖状态、Rt-PCR和Western blot等检测Akt和p-Akt表达以及放射同位素法检测MSCs对氚标-葡萄糖（^3H-G）的摄取等。结果1.Akt基因显著降低MSCs缺氧时AR和DR（P〈0.01）,而各缺氧时间点没有统计学意义（P〉0.05）;2.Akt基因显著增高MSCs常氧和缺氧（与未转染Akt基因MSCs同等条件下比较）时增殖能力（P〈0.01）,缺氧时增殖能力显著低于常氧时（P〈0.01）;3.Akt基因显著增高常氧时MSCsAkt mRNA（P〈0.01）和蛋白（P〈0.01）表达,而不增高p-Akt蛋白（P〉0.05）表达;Akt基因显著提高缺氧时p-Akt蛋白（P〈0.01）表达,而不提高常氧时p-Akt蛋白（P〉0.05）表达;4.Akt基因显著增高MSCs常氧和缺氧（与未转染Akt基因MSCs同等条件下比较）时^3H-G的摄取（P〈0.01）,缺氧时^3H-G的摄取显著性低于常氧培养时（P〈0.01）;^3H-G的摄取与细胞增殖显著正相关（r=0.79,P=0.015）而与细胞凋亡显著负相关（r=-1.47,P=0.023）。结论Akt基因转染可显著提高MSCs耐缺氧能力,此可能与缺氧时改善MSCs葡萄糖摄取等有关。     

RESPONSE OF MOUSE BONE MARROW COLONY FORMING UNITS IN DIFFERENT STAGES OF THE CELL CYCLE TO IN VITRO INCUBATION WITH MITOMYCIN-C

A short-term in vitro method was employed to study the Mitomycin-C sensitivity of normal mouse bone marrow CFU without triggering the G₀-phase cells into the proliferative cycle. Comparison was made of the toxicities of the drug against cells in different phases of the cell cycle including G₀. Mitomycin-c killed CFU both in and out of the S-phase. No significant difference could be found between its toxicities against normal and proliferating CFU; along the exponential part of the survival curve 1·6 μg/ml concentration of the drug reduced survival to 10%. Although in the normal bone marrow only a few CFU are in the S-phase and are killed by the agent, presence of the sensitive G₀ cells produce a significant amount of non-S-phase mortality. Among the proliferating CFU population the non-S-phase lethality is less due to the absence of G₀ cells. About 75% of the S-phase cells are killed after incubation with 1 μg/ml drug; outside the S-phase, the lethality is about 40–50%. The studies indicate that the G₀ cells which are situated near the G₁-S boundary are almost as sensitive to the drug as other non-S-phase cells like G₁ cells. The clinical significance of the findings is discussed.     

PROLIFERATION OF ERYTHROID AND GRANULOCYTE PROGENITORS IN THE SPLEEN AS A FUNCTION OF STEM CELL DOSE

A study of the kinetics of cellular proliferation, in the morphologically unrecognizable haemopoietic progenitor cell compartment, as a function of injected CFU-S dose has been carried out in the spleens of lethally X-irradiated mice using ³H-TdR labelling. Amplification in this proliferating cell compartment was observed to decline as CFU-S dose increased. The number of divisions in the differentiated line arising from CFU-S up to the first appearance of recognizable erythroid precursors were calculated to be 9.2, 12.5, 15 and 17 for the 2, 0.35, 0.05 and 0.007 femur equivalent doses respectively. The growth of cell populations arising from CFU-S was biphasic, with a rapid initial phase having a doubling time of about 6.3 hr, and a slow phase of doubling time around 1 day. Analysis of the rapid phase by the FLM method gave a cycle time of 5.6 hr. Recognizable labelled erythroid precursors were detected at the same time as, or just after, the change in slope of the growth curve. Significant numbers of proliferating (labelled) granulocytes only appeared in the spleens of animals receiving the higher marrow doses (2 and 0.35 femur). The erythroid to granulocyte ratio was also a decreasing function of marrow dose.     

骨髓动员对骨髓造血干细胞在心肌梗死后心脏中定植及分化的影响

目的观察小鼠心肌梗死后骨髓造血干细胞在心脏内的分化及细胞因子的影响。方法C57/BL6小鼠60只分为骨髓动员组和对照组,先后行脾切除、骨髓移植（骨髓供体为增强绿色荧光蛋白转基因小鼠）、骨髓动员及建立心肌梗死模型。心肌梗死后3周将小鼠心脏取出并切片行组织学及激光共聚焦显微镜免疫荧光检查。结果骨髓动员可以增加EGFP阳性细胞在心脏中梗死区和边缘区的定植,但绝大多数EGFP阳性细胞都同时表达CD45。仅发现有极少数骨髓来源的心肌细胞、成纤维细胞及血管内皮细胞,且与骨髓动员无相关性。结论骨髓动员能够明显促进骨髓来源细胞定植入小鼠心脏的梗死区;极少数骨髓造血干细胞可以分化为心肌细胞,其数量远不足以修复梗死心肌及改善心功能;骨髓造血干细胞不参与梗死区疤痕形成的病理过程。     

骨髓基质干细胞向心肌细胞诱导分化的实验研究

目的探讨大鼠骨髓基质干细胞在体外和体内向心肌细胞诱导分化的能力,为下一步的细胞移植治疗心肌梗死提供实验基础.方法体外诱导实验中,将不同浓度的5-氮胞苷作用于不同培养时间的骨髓基质干细胞,摸索5-氮胞苷的最佳诱导时机和浓度,观察诱导后细胞形态变化,并用免疫细胞化学染色检测心肌特异性肌钙蛋白T的表达;在体内实验中,培养扩增的骨髓基质干细胞经BrdU标记后,自体移植于正常心肌内,分别通过BrdU和心肌特异性肌钙蛋白T免疫组织化学染色检测移植细胞的存活和分化情况.结果体外诱导实验中,5-氮胞苷的诱导作用以10μmol/L的浓度对传代细胞进行两次诱导,效果最好,不仅能诱导出表达心肌特异蛋白的心肌样细胞,而且这些细胞在体外能够自发搏动.体内诱导实验中,移植的细胞在正常心肌微环境中能够存活并分化为心肌细胞.结论骨髓基质干细胞在体外化学诱导和体内心肌微环境诱导时均能分化为心肌细胞,可用于细胞移植治疗心肌梗死的实验.     

RADIOAUTOGRAPHIC STUDIES OF THE STEM CELL IN THE THYMUS OF THE IRRADIATED RAT

Radioautographic evidence is presented which characterizes the marrow derived stem cell which promotes thymic recovery following irradiation in the rat. These immigrant cells are similar in morphology to blood monocytes and have been called monocytoid, meaning monocyte-like in appearance. The typical cell had abundant pale staining cytoplasm and a nucleus with many invaginations and folds and a fine chromatin structure. There was no prominent nucleolus. The majority of these cells entered the thymus of the irradiated rat via the blood vessels into the septa and made their way through the connective tissue to the outer cortex. Three distinct morphological cell types appeared to be derived from the immigrant cells. These were fibrocyte-like cells which were located within the septa, macrophages located mainly within the medulla and septa, and large blast cells within the cortex, which proliferated giving rise to large thymocytes. The blast cells were characterized as having abundant moderately basophilic (and pyroninophilic) cytoplasm with a distinct cytoplasmic boundary, a large nucleus which still had invaginations and folds, a loose chromatin structure and one or more very prominent nucleoli. They were located in groups primarily within the outer cortex and often adjacent to blood vessels. They were found to be highly susceptible to damage in smear preparations. In contrast, their progeny, the large thymocytes were not highly susceptible to damage in smear preparations but teased out as large round cells with a highly basophilic rim of cytoplasm. The large thymocytes were precursors to medium and small cells. A radioautographic technique for 1 μ tissue sections is also described.     

DYNAMIC HISTOLOGY OF A RAT HEPATOMA AND THE RESPONSE TO 5-FLUOROURACIL*

The cellular response of the rat hepatoma 3924A to a single intraperitoneal injection of 5-fluorouracil has been measured in respect of the spatial relationship of the cells to the tumour microvasculature. In this tumour the parenchyma is arranged in cords approximately 150 μm thick around central capillaries. For untreated tumours, those cells at distances less than 80 μm from the capillary had a mean [³H]TdR labelling index of 39% and a mitotic index of 2·1%, while for those cells more than 80 μm away the values were 14% and 0·8% respectively. Two days after 150 mg/kg of 5-fluorouracil, mean cord thickness was reduced by 25% and did not recover to the control level until 11 days after treatment. This was also true for the mitotic index. Recovery of the labelling index was complete 2 days earlier. Although absolute values of parameters were different in the populations adjacent to and remote from the capillary, the time course of recovery was similar, with a ‘growth spurt’ 7 to 9 days after treatment. The results from this histologically-based assay have been compared with those from biochemical/biophysical assays that sample the overall tumour population.     

THE INFLUENCE of A LOW ENVIRONMENTAL TEMPERATURE ON the STEM CELL POPULATION of the BONE MARROW and INTESTINAL MUCOSA

Protracted exposure of rats to a low environmental temperature (2° C) resulted in almost a two-fold increase in the number of colony forming units per femur. Following a dose of Vinblastine, return of CFUs in the bone marrow to the pretreatment level was more rapid in the cold exposed rats than in rats at a 25° C environment. the cell cycle time of the cells in the intestinal crypt was reduced for the cold exposed rats. These observations are thought to be the basis for the increased radioresistance and/or more rapid recovery from whole body irradiation previously reported.     

泽蛙(Rana limnocharis)活体内骨髓细胞增殖动力学的研究

离体培养的动物细胞增殖规律已有不少的报道,但是两栖类活体内细胞增殖过程如何,尚未见报道。本文运用SCD术,对泽蛙活体内骨髓细胞增殖动力学进行了较系统地观察,最后推算出Tc为12—24小时。     

小鼠骨髓内皮细胞无血清条件培养液及其超滤组分对粒巨噬系祖细胞生长的影响

本研究通过传代培养小鼠骨髓内皮细胞系细胞,收集无血清条件培养液(mBMECCM),将其作多级串联超滤,获得分子量大于10、3～10、1～3、05～1kD和小于05kD超滤组分。进行粒巨噬系造血祖细胞集落形成试验,检测了它们的作用。mBMECCM和3～10kD组分对粒巨噬系祖细胞(CFUGM)生长未见明显影响,而分子量大于10kD和05～1kD组分促进CFUGM的增殖,分子量1～3kD和小于05kD组分则抑制CFUGM的增殖。这4种超滤组分对CFUGM生长的效应均有剂量依赖性。这些结果提示,在体外培养条件下,小鼠骨髓内皮细胞分泌若干种活性成分,分别对CFUGM的生长起促进或抑制作用     

大鼠骨髓间充质干细胞的分离纯化与初步鉴定

目的：探讨体外分离、纯化大鼠骨髓间充质干细胞(mesenchymal stem cells,MSCs)的方法,分析其部分表型特点。方法：用密度梯度离心结合贴壁培养法分离纯化大鼠骨髓MSCs,传代扩增,测定生长曲线,形态学观察,免疫细胞化学及图像分析测定细胞表面抗原和细胞外基质蛋白表达情况。结果：MSCs属骨髓中单个核细胞,密度梯度离心结合贴壁培养法能有效分离纯化大鼠骨髓MSCs,MSCs在含10％小牛血清的L-DMEM中生长性状相对稳定,1、3、5代细胞生长曲线基本一致,增殖速度快。细胞呈均一的成纤维细胞样,均一表达CD44、CD54、纤维粘连蛋白(Fibronectin,FN)、Ⅰ型胶原(CollagenⅠ)。结论：本实验建立了一种体外分离纯化、培养扩增大鼠骨髓MSCs的方法,MSCs稳定表达CD44、CD54、FN、CollagenⅠ。     

THE EFFECT OF POLYCYTHAEMIC SERUM ON THE PROLIFERATION OF RAT BONE MARROW CELLS IN VITRO

The effect of experimental polycythaemia on the rate of proliferation of erythrocytic precursor cells was investigated by means of an in vitro technique. The serum obtained from polycythaemic rats was found to inhibit significantly ³H-thymidine incorporation in normal rat bone marrow cells in vitro, as compared with normal serum. Autoradiographic analysis revealed that this inhibition resulted from a reduction in the number of labelled bone marrow cells. The inhibition proved to be specific to the erythrocyte precursor cells; the labelling index was reduced in the erythrocytic cell population by 21–50% (P < 0.001) at different incubation times, while the effect on the granulocytic cell population was negligible. It is deduced that an inhibitor substance responsible for the effects observed is present in polycythaemic serum. It is proposed that this factor is the ‘erythrocytic chalone'. The results support the general view that triggering of stem cells is not the only mode of regulation of erythropoiesis, but that the rate of proliferation of the precursor cells in the erythron is also regulated.     

EFFECT OF CYCLOPHOSPHAMIDE ON THE HEMATOPOIETIC MICROENVIRONMENTAL FACTORS WHICH INFLUENCE HEMATOPOIETIC STEM CELL PROLIFERATION

Transplanted hematopoietic stem cells (HSC) regenerate more rapidly in the femoral marrow of lethally irradiated hosts pretreated with cyclophosphamide (CY) 4 days prior to X-irradiation than they do in that of uninjected irradiated hosts (control). On the other hand, regeneration of HSC transplanted into irradiated hosts given CY 7 days before X-irradiation is slower than in controls.
The microenvironment in the femoral marrow was studied at various times after giving CY. Four days after injecting CY, the number of colony forming units (CFU), total nucleated hematopoietic cells, and mature myeloid and erythroid cells in the femoral marrow is markedly reduced. Seven days after injecting CY, the number of CFU in the femoral marrow is still reduced, the total nucleated cell count is back to normal, but the number of mature myeloid elements in the marrow are significantly increased. These observations suggest the conclusion that the rate of proliferation of HSC is modulated by the number of mature myeloid cells in the microenvironment.     

MULTIPLICATION OF HAEMOPOIETIC COLONY FORMING UNITS (CFU) IN MICE AFTER X-IRRADIATION AND BONE MARROW TRANSPLANTATION

Kinetics of the multiplication of haemopoietic CFUs was studied in lethally irradiated mice receiving various numbers of syngeneic bone marrow cells. After transplantation of a small number of bone marrow cells, the growth rate of CFU in femoral bone marrow appeared to decrease after about 10 days after transplantation, before the normal level of CFU in the femur was attained. In the spleen it was found that the overshoot which was observed about 10 days after transplantation of a large number of bone marrow cells is smaller or absent when a small number of cells is transplanted. Experiments dealing with transplantation of 50 x 10⁶ bone marrow cells 0, 4 or 10 days after a lethal irradiation indicated that the decline in growth rate of CFUs about 10 days after irradiation could not be attributed to environmental changes in the host.
The results are explained by the hypothesis that a previous excessive proliferation of CFUs diminishes the growth rate thereafter. This hypothesis is supported by experiments in which 50 x 10⁶ bone marrow cells derived from normal mice or from syngeneic chimaeras were transplanted. The slowest growth rate was observed when bone marrow that had been subjected to the most excessive proliferation in the weeks preceding the experiment was transplanted.     

THE ENHANCEMENT OF HAEMOPOIETIC STEM CELL RECOVERY IN IRRADIATED MICE BY PRIOR TREATMENT WITH CYCLOPHOSPHAMIDE

Studies are reported of the enhancement of stem cell recovery following whole body irradiation as a result of prior administration of cyclophosphamide. It is shown that the much larger enhancement of regeneration observed for the hosts own surviving stem cells, compared to the regeneration of injected bone marrow stem cells, is due to the different numbers of stem cells initiating the regeneration in conjunction with the time course of stem cell regeneration. The results show that the environmental changes produced by cyclophosphamide greatly enhance haemopoietic recovery even though at the dose used this agent is relatively toxic to stem cells. Furthermore it has been shown that the level of stem cell regeneration is nearly independent of the γ-ray dose in the range 3–8 gray (300–800 rad). If human bone marrow should respond similarly it follows that regeneration produced by cytotoxic drugs administered prior to radiation embodies a considerable safety factor as far as recovery of the haemopoietic system is concerned.