远红外线对造血干/祖细胞生物学特性的影响

目的:了解远红外线对造血细胞增殖和定向分化的影响.方法:应用体外小鼠骨髓细胞培养技术,观察远红外线对拉-单祖细胞(CFU-GM),红系祖细胞(CFU-E)和成纤维细胞(CFU-F)增殖和分化的影响,并且利用免疫荧光纳米粒子(1FNB)检测靶细胞表面分化抗原(CD),进一步评佑远红外线对造血干/祖细胞的影响.结果:远红外线在37℃条件下照射时CFU-E、CFU-F和CFU-GM生成有促进作用,小鼠骨髓细胞表面标记有变化,靶细胞经2min照射后,增殖最旺盛.2min组与其它实验组(1min,5min,10min)数据经统计学处理,具有差异性(P均<0.05).结论:远红外线时小鼠骨髓造血干/祖细胞的增殖具有正调节作用并可诱导细胞表面标志改变.     

口服携带人PF4基因的减毒沙门氏菌对大剂量化疗小鼠的促造血重建作用

目的:探索口服携带人PF4基因的减毒沙门氏菌对大剂量化疗小鼠造血重建作用。方法:通过在大剂量化疗前／后喂服携带PIRES2-EGFP／PF4减毒沙门氏菌,检测化疗后小鼠的生存率,小鼠在不同时间外周血血常规、骨髓细胞数、骨髓中Sca-1和C-kit细胞含量、不同时间骨髓生成各系细胞的集落数等。结果:在大剂量化疗前、后均口服携带PIRES2-EGFP／PF4减毒沙门氏菌组小鼠生存率高于只在化疗前口服携带PIRES2-EGFP／PF4减毒沙门氏菌组;两组口服携带PIRES2-EGFP／PF4减毒沙门氏菌组小鼠存活率明显高于PBS对照组及携带空载体的减毒沙门氏菌组;口服携带PIRES2-EGFP／PF4减毒沙门氏菌组小鼠在化疗后第9~12天的外周血血小板数、骨髓细胞中Sca-1和C-kit阳性细胞含量明显比对照组高,第5天、9天、12天的骨髓细胞总数、骨髓细胞形成Mix集落数明显增加。结论:口服减毒沙门氏菌SL3261为载体的PF4基因可以保护小鼠免受损伤,并促进化疗损伤小鼠的造血恢复。     

白介素3治疗小鼠造血功能低下的疗效及机理初探

通过整体实验观察国产重组白介素３（ＩＬ－３）对射线和环磷酰胺所致小鼠造血功能低下的疗效;以体外实验分析其疗效机理。实验结果表明：（１）ｒｈＩＬ－３腹腔或皮下连续５天注射能全面提高７Ｇｙ照射小鼠９天时股骨骨髓ＣＦＵ－Ｅ、ＢＦＵ－Ｅ、ＣＦＵ－Ｍｉｘ和ＣＦＵ－ＧＭ的产率和数量,其效果强弱与注射途径和用药剂量有关。ｒｈＩＬ－３对小鼠股骨骨髓有核细胞总数和内源性脾结节数的改善影响小。（２）ｒｈＩＬ－３对环磷酰胺所致小鼠造血功能低下亦有改善效果,并与起用时间和剂量有关。（３）ｒｈＩＬ－３对人骨髓细胞和ＣＦＵ－ＧＭ集落形成有明显的增强作用。小鼠骨髓细胞对ｒｈＩＬ－３缺乏反应;对ｒｍＩＬ－３有增殖分化加强的反应。ｒｍＩＬ－３体外共育能提高正常及照射２Ｇｙ小鼠骨髓细胞体外培养后ＣＦＵ－ＧＭ的产率和数量。文中讨论了ＩＬ－３的应用前景及合理方案问题。     

Exo-1基因对端粒酶缺陷小鼠造血干细胞植入效率的影响

目的利用不同的造血干细胞移植方式,探讨Exo-1基因缺失对端粒酶基因敲除小鼠的造血干细胞植入效率的影响。方法以CD45.1小鼠的骨髓细胞或骨髓造血干细胞为供体,以端粒酶基因敲除小鼠或Exo-1基因和端粒酶基因双敲除小鼠为受体,在给予不同剂量X线照射或不照射的情况下,重复进行静脉注射全骨髓细胞或分选的骨髓造血干细胞(c-kit+、Sca-1+、lineage-,KSL),于移植后1个月取外周血,流式分析嵌合率。结果未经X线照射及1 Gy、2 Gy照射情况下,端粒酶基因缺陷受体小鼠的外周血中供体来源的细胞嵌合率较低;6 Gy照射后,供体来源的外周血细胞嵌合率仍低于50%,而且端粒酶基因缺陷受体小鼠在移植后1个月内死亡较多;3 Gy照射可形成较高嵌合率,Exo-1基因缺失对端粒酶缺陷小鼠的造血干细胞植入效率的影响不显著。结论以端粒酶缺陷小鼠作为衰老模型研究造血干细胞植入效率时,3 Gy X线照射能够有效地形成较高的外周血供体细胞的嵌合率,但是Exo-1基因没有进一步提高造血干细胞在端粒酶敲除小鼠的植入效率。     

p18INK4C基因缺失增强造血干细胞在亚致死剂量照射小鼠体内长期植入能力

观察p18INK4C(p18)基因缺失对造血干细胞(HSC)在亚致死剂量照射小鼠体内长期植入的影响. 供体为p18基因缺失型(p18(/()纯系C57BL/6小鼠(CD45.2表型), 竞争性细胞来源于C57BL/6-Ly5.1(CD45.1/2)双表型小鼠, 受体为野生型(p18+/+)C57BL/6-Ly5.1(CD45.1)小鼠. 竞争性骨髓移植(cBMT)实验根据受体小鼠照射剂量的不同分为3个剂量组(10 Gy, 5 Gy和1 Gy). 供体细胞和竞争性细胞1:1混合后移植, 移植后采集外周血和骨髓细胞用流式细胞仪检测各细胞比例. 造血恢复移植实验: 移植后检测外周血白细胞计数评价移植后造血恢复速度. 10和5 Gy照射剂量组, 供体细胞和竞争性细胞成功植入, 而1 Gy照射剂量组无供体细胞植入. 无论在10 Gy或是5 Gy照射剂量情况下, 供体细胞在受体内的比例均高于竞争性细胞. 移植后6周, 10和5 Gy照射剂量时外周血中供体细胞比例分别为竞争性细胞的1.46±0.21倍和1.64±0.43倍, 14周时分别为竞争性细胞的1.84±0.25倍和2.00±0.49倍, 26周时分别为竞争性细胞的3.13±0.79倍和3.24±1.33倍. 移植后6个月, 10 Gy照射剂量时骨髓细胞中供体细胞比例为竞争性细胞的7.68±4.42倍, 5 Gy照射剂量时为竞争性细胞的10.83±2.98倍. 移植后6个月, 在10和5 Gy照射剂量组之间骨髓中造血细胞植入率相当, 分别为(85.53±8.71)%和(80.87±2.87)% (P = 0.457). p18(/(细胞与p18+/+细胞相比, 移植后造血恢复的速度相当. p18基因缺失可以显著增强HSC在亚致死剂量照射小鼠体内的长期植入能力.     

小分子化合物Me6TREN促进小鼠骨髓中造血干/祖细胞的增殖

目的:探讨小分子化合物Me6TREN对小鼠骨髓中造血干/祖细胞的增殖作用。方法:采用细胞计数、细胞集落形成能力检测、流式细胞术检测细胞表面标志等实验技术,观察Me6TREN对小鼠骨髓细胞的影响。结果:皮下注射Me6TREN 12 h后,Me6TREN组的集落形成能力、造血干/祖细胞表面标志lin-Sca-1+c-Kit+的比例均明显高于对照组;在体外分离培养的小鼠骨髓单个核细胞,4 d后Me6TREN组细胞的集落形成能力及造血干/祖细胞的增殖能力均高于对照组。结论:Me6TREN对小鼠骨髓造血干/祖细胞有一定的促增殖作用。     

天然杀伤细胞在受照射小鼠中的造血调控作用

研究了天然杀伤（ＮＫ）细胞对受致死剂量γ线照射的同系小鼠的造血调控作用。ＡＭＳ／５小鼠经９Ｇｙγ线全身照射后立即经尾静脉注射ＮＫ细胞（５×１０５）,可明显提高受照小鼠３０ｄ活存率,照后８ｄ小鼠骨髓中ＣＦＵ－ＧＭ数量明显高于对照和脾细胞注射组,照射后３０ｄ,ＮＫ细胞注射组活存小鼠的骨髓有核细胞数和ＣＦＵ－ＧＭ数已恢复到正常的７６％─９６％。病理组织学观察显示,输注ＮＫ细胞可使小鼠骨髓、脾脏的组织损伤程度减轻,造血功能增强,表现为造血灶数增多,造血细胞功能活跃,核分裂相增多,且涉及红系、粒系、巨核细胞系造血。ＮＫ细胞可能通过直接与造血干细胞相互作用或改善造血微环境等促进“内源性”造血功能,从而发挥对造血的正调控作用。提示ＮＫ细胞在小鼠造血功能的平衡维持中起重要作用。     

CD34+和CD34-细胞在NOD/SCID小鼠体内的造血重建

利用非肥胖糖尿病型重症联合免疫缺陷型(NOD/SCID)小鼠模型, 比较了新鲜及培养后的CD34+和CD34-细胞在体内植入及重建造血能力。从新鲜脐血及培养后的单个核细胞(MNC)中分离出CD34+和CD34-细胞, 经尾静脉输注入经亚致死剂量照射的NOD/SCID小鼠体内, 6周后处死存活的小鼠, 取其骨髓、脾脏和外周血细胞, 分别进行细胞表型分析、造血集落形成单位和人特异性基因的检测。经检测, 输注CD34+细胞和混合细胞的小鼠, 其体内CD45+细胞及人源各系血细胞的含量相近, 两者均远远高于输注CD34-细胞的小鼠。输注培养后CD34-细胞的小鼠饲养6周后全部死亡,输注培养后CD34+细胞的小鼠存活率约为66.7%, 而输注培养后混合细胞的小鼠全部存活, 且在两组存活的小鼠体内均能检测到CD45+细胞及人源各系血细胞。结果表明: 无论是新鲜还是培养后的CD34+细胞均具有在NOD/SCID小鼠体内植入和重建造血能力, 而CD34-细胞不具有该能力, 但CD34-细胞与CD34+细胞同时输注有助于提高小鼠的存活率, 说明其对CD34+细胞在小鼠体内发挥植入和造血重建能力有一定的辅助作用。     

人CD34^＋和CD34^-细胞在NOD／SCID小鼠体内的造血重建

利用非肥胖糖尿病型重症联合免疫缺陷型(NOD/SCID)小鼠模型,比较了新鲜及培养后的CD34 和CD34-细胞在体内植入及重建造血能力.从新鲜脐血及培养后的单个核细胞(MNC)中分离出CD34 和CD34-细胞,经尾静脉输注入经亚致死剂量照射的NOD/SCID小鼠体内,6周后处死存活的小鼠,取其骨髓、脾脏和外周血细胞,分别进行细胞表型分析、造血集落形成单位和人特异性基因的检测.经检测,输注CD34' 细胞和混合细胞的小鼠,其体内CD45 细胞及人源各系血细胞的含量相近,两者均远远高于输注CD34-细胞的小鼠.输注培养后CD34-细胞的小鼠饲养6周后全部死亡,输注培养后CD34 细胞的小鼠存活率约为66.7%,而输注培养后混合细胞的小鼠全部存活,且在两组存活的小鼠体内均能检测到CD45 细胞及人源各系血细胞.结果表明:无论是新鲜还是培养后的CD34 细胞均具有在NOD/SCID小鼠体内植入和重建造血能力,而CD34-细胞不具有该能力,但CD34-细胞与CD34 细胞同时输注有助于提高小鼠的存活率,说明其对CD34 细胞在小鼠体内发挥植入和造血重建能力有一定的辅助作用.     

大豆异黄酮对辐射小鼠造血系统损伤防护作用的实验研究

研究大豆异黄酮(SoybeanIsoflavone,SI)对辐射损伤小鼠造血系统功能的影响。雄性昆明小鼠照射前补充SI,经4Gyγ射线照射,观察补充SI对电离辐射损伤小鼠内源性脾结节(CFU-S)数、骨髓细胞粒、巨噬系细胞集落形成单位(CFU-GM)数、骨髓细胞DNA含量及外周血淋巴细胞DNA损伤程度的影响。结果显示SI提高了辐射损伤小鼠CFU-S数,增加了骨髓有核细胞CFU-GM数,降低外周血淋巴细胞DNA损伤程度,对骨髓细胞DNA含量也有一定的增加趋势。表明SI可以提高辐射损伤小鼠造血干祖细胞的增殖能力,减轻辐射对骨髓细胞和外周血淋巴细胞DNA的损害,SI对辐射小鼠的造血系统有一定的防护作用。     

载氢-纳米氧化铈微泡对小鼠造血系统抗辐射作用的分析

为探讨载氢-纳米氧化铈微泡对小鼠辐射损伤的防护作用。本研究检测载氢-纳米氧化铈微泡的表征,并将60只BALB/c小鼠随机分为正常对照组、照射对照组、载氢-纳米氧化铈微泡组。小鼠经6Gy x射线一次性全身照射(剂量率2 Gy/min)。于照射后3 d和8 d处死小鼠,检测其外周血细胞数、脾脏和胸腺指数、骨髓和脾脏组织病理学变化。结果显示,照射后3 d和8 d,与正常对照组相比,载氢-纳米氧化铈微泡组和照射对照组的白细胞均明显下降,相比照射对照组,载氢-纳米氧化铈微泡组有改善(p<0.05或p<0.01);而载氢-纳米氧化铈微泡组和照射对照组的红细胞数和血红蛋白均略有下降,但差异无统计学意义。与正常对照组相比,微泡组的胸腺指数、脾脏指数均有下降,和照射对照组相比,载氢-纳米氧化铈微泡组的胸腺指数明显改善(p<0.05或p<0.01)。照射后3 d,与正常对照组相比,照射对照组的骨髓细胞较少,存在细胞碎片,载氢-纳米氧化铈微泡组骨髓细胞数量略有减少,存在细胞核松散现象。而照射后8 d,与正常对照组相比,照射对照组的骨髓细胞几乎找不到,载氢-纳米氧化铈微泡组骨髓细胞有一定数量,存在细胞凋亡现象。本研究表明,载氢-纳米氧化铈微泡通过保护造血组织、改善造血功能,对机体起到一定的辐射防护作用。     

Bone marrow-derived T lymphocytes responsible for allograft rejection

Lethally irradiated mice reconstituted with syngeneic bone marrow cells were grafted with allogeneic skin grafts 6-7 weeks after irradiation and reconstitution. Mice with intact thymuses rejected the grafts whereas the mice thymectomized before irradiation and reconstitution did not. Thymectomized irradiated mice (TIR mice) reconstituted with bone marrow cells from donors immune to the allografts rejected the grafts. Bone marrow cells from immunized donors, pretreated with Thy 1.2 antibody and C', did not confer immunity to TIR recipients. To determine the number of T lymphocytes necessary for the transfer of immunity by bone marrow cells from immunized donors, thymectomized irradiated mice were reconstituted with nonimmune bone marrow cells treated with Thy 1.2 antibody and C' and with various numbers of splenic T lymphocytes from nonimmune and immune donors. Allogeneic skin graft rejection was obtained with 10(6) nonimmune or 10(4) immune T cells. The effect of immune T cells was specific: i.e., immune T cells accelerated only rejection of the relevant skin grafts whereas against a third-party skin grafts acted as normal T lymphocytes.     

Effect of graft-versus-host disease (GVHD) on host hematopoietic progenitor cells is mediated by Fas-Fas ligand interactions but this does not explain the effect of GVHD on donor cells.

The acute graft-versus-host disease (GVHD) generated in BDF1 mice by the injection of spleen cells from the C57BL/6 parental strain induces a direct cell-mediated attack on host lymphohematopoietic populations, resulting in the reconstitution of the host with donor hematopoietic stem cells. We examined the effect of GVHD on the donor and host hematopoiesis in parental-induced acute GVHD. The bone marrow was hypoplastic and the number of hematopoietic progenitor cells significantly decreased at 4 weeks after GVHD induction. However, extramedullary splenic hematopoiesis was present and the number of hematopoietic progenitor cells in the spleen significantly increased at this time. Fas expression on the host spleen cells and bone marrow cells significantly increased during weeks 2 to 8 of GVHD. Host cell incubation with anti-Fas Ab induced apoptosis, and the number of hematopoietic progenitor cells decreased during these weeks. A significant correlation between the augmented Fas expression on host bone marrow cells and the decreased number of host bone marrow cells by acute GVHD was observed. Furthermore, the injection of Fas ligand (FasL)-deficient B6/gld spleen cells failed to affect host bone marrow cells. Although Fas expression on repopulating donor cells also increased, Fas-induced apoptosis by the repopulating donor cells was not remarkable until 12 weeks, when more than 90% of the cells were donor cells. The number of hematopoietic progenitor cells in the bone marrow and the spleen by the repopulating donor cells, however, decreased over an extended time during acute GVHD. This suggests that Fas-FasL interactions may regulate suppression of host hematopoietic cells but not of donor hematopoietic cells. Hematopoietic dysfunctions caused by the reconstituted donor cells are independent to Fas-FasL interactions and persisted for a long time during parental-induced acute GVHD.     

骨髓移植小鼠二甲基亚硝胺肝纤维化模型的建立

目的构建绿色荧光蛋白(GFP)标记骨髓细胞的小鼠,并复制其二甲基亚硝胺(DMN)肝纤维化模型。方法 ICR雄性小鼠32只,随机分为正常组6只和移植组26只。移植组接受致死量γ射线照射后,经尾静脉输入GFP转基因小鼠的骨髓细胞;正常组不进行照射和移植,仅尾静脉注射等量生理盐水。两个月后制备血涂片,观察移植组造血重建情况,造血重建动物再分为对照组和造模组,造模组用DMN按每次10mg/kg体重腹腔注射制备肝纤维化模型,隔日一次,正常组和对照组给予等量生理盐水。设染毒后3周和4周两个时间观察点,生化法测定肝功能;Jamall法检测肝组织羟脯氨酸含量;HE染色及天狼猩红染色观察肝组织炎症、坏死及纤维组织增生情况;GFP免疫荧光组织化学观察骨髓源性细胞在肝脏的归巢特点。结果骨髓移植两个月后,移植组外周血中出现满视野GFP+细胞。与正常组比较,两个时间观察点造模组肝功能(ALT、AST、Alb及T.Bil)均明显异常(P<0.05),肝组织羟脯氨酸含量显著增高(P<0.05),造模3周末肝组织出血性坏死,有炎性细胞浸润,但尚未形成完全的纤维间隔;造模4周末肝组织炎症、坏死程度加重,可见完全的纤维间隔,在DMN造模动物肝组...     

Use of flt3 ligand to evaluate residual hematopoiesis after heterogeneous irradiation in mice

We evaluated the possibility of using plasma Flt3 ligand (FL) concentration as a biological indicator of bone marrow function after heterogeneous irradiation. Mice were irradiated with 4, 7.5 or 11 Gy with 25, 50, 75 or 100% of the bone marrow in the field of irradiation. This model of irradiation resulted in graded and controlled damage to the bone marrow. Mice exhibited a pancytopenia correlated with both the radiation dose and the percentage of bone marrow irradiated. The FL concentration in the blood increased with the severity of bone marrow aplasia. Nonlinear regression analysis showed that the FL concentration was strongly correlated with the total number of residual colony-forming cells 3 days after irradiation, allowing a precise estimate of residual hematopoiesis. Moreover, the FL concentration on day 3 postirradiation was correlated with the duration and severity of subsequent pancytopenia, suggesting that variations in FL concentrations might be used as a predictive indicator of bone marrow aplasia, especially by the use of linear regression equations describing these correlations. Our results provide a rationale for the use of FL concentration as a biological indicator of residual hematopoiesis after heterogeneous irradiation.     

Cellular events during radiation-induced thymic leukemogenesis in mice: abnormal T cell differentiation in the thymus and defect of thymocyte precursors in the bone marrow after split-dose irradiation

Cellular events during the development of thymic lymphomas in young B10.BR mice given leukemogenic split-dose irradiation were studied by examining the differentiation of functional T lymphocyte precursors in the regenerating thymus. It was found that leukemogenic radiation treatment resulted in a sustained depression of the level of thymic cytotoxic T lymphocyte precursors (CTLp) and of mixed lymphocyte reactivity of thymus cells when assessed between 1 and 4 mo after irradiation, in spite of the fact that the total number of thymocytes was restored to the normal level within 2 mo and continued to increase thereafter. In vitro mixing studies of normal thymocytes with thymus cells from split-dose irradiated mice provided no evidence for active suppression as a mechanism for this depressed activity. The ability of bone marrow cells from split-dose irradiated mice to regenerate the thymus and to differentiate into functional CTLp was examined by use of supralethally irradiated Thy-1 congenic recipients. Reconstitution of supralethally irradiated B10.BR Thy-1.2 mice with normal bone marrow from B10.BR Thy-1.1 mice resulted in the complete repopulation of host-thymus with donor-derived cells when assessed at 4 wk after reconstitution. Lymphocytes from the regenerating thymus of these animals were shown to contain high levels of CTLp which were donor-derived. On the other hand, when the recipient mice were reconstituted with bone marrow cells from donor mice which had been split-dose irradiated 1 mo earlier, regeneration of the recipient thymus was severely depressed when assessed at 4 wk to 3 mo after reconstitution. Although variable but small numbers of donor-derived Thy-1+ cells were detected, CTL activity for alloantigen could not be induced in these donor-derived cells. The results suggest that T cell precursors derived from split-dose irradiated donor mice were unable to undergo active proliferation and differentiation into functional CTLp. The significance of these findings on radiation-induced thymic leukemogenesis is discussed.     

Effect of 2450 MHz microwave radiation on hematopoiesis of pregnant mice

In this study, the influence of 2450 MHz CW microwave radiation on hematopoiesis in pregnant mice was examined. Dams (mice CD-1 strain) were irradiated during Days 1-6 or 6-15 of pregnancy. The animals were irradiated for a total of 8 hr per day (two 4-hr exposures in 9 hr) at an average power density of 30 mW/cm2. Peripheral blood and bone marrow samples were obtained on Day 18 of pregnancy. The total leukocyte and differential leukocyte counts of peripheral blood samples were not affected by either exposure regimen. In addition, no effects were noted in either the erythroid or myeloid mitotic indices of bone marrow samples. Exposure of pregnant mice to microwave radiation under the conditions of these experiments had no effects on the investigated aspects of hematopoiesis.     

Full reconstitution of the immune deficiency in scid mice with normal stem cells requires low-dose irradiation of the recipients

Mice homozygous for an autosomal recessive mutation for the scid gene exhibit a defect that specifically impairs lymphoid differentiation but not myelopoiesis. Such mice can be cured of their lymphoid deficiency by grafts with normal bone marrow, although full reconstitution of lymphoid function is seldom obtained. Long-term bone marrow cultures (LTBMC) are devoid of all mature B and pre-B cells but contain lymphoid stem cells. We therefore reconstituted scid mice with LTBMC cells to study the kinetics of B lymphocyte reconstitution in normal and irradiated (4 Gy) scid recipients and in irradiated (9.5 Gy) co-isogenic C.B-17 mice. Detectable colony-forming B cells rapidly increased in the spleen and bone marrow of irradiated C.B-17 and irradiated scid recipients, reaching normal levels between 4 and 6 wk post-grafting. Unirradiated scid recipients showed limited reconstitution in spleen and very poor reconstitution in bone marrow. Unirradiated scid recipients also had relatively few surface Ig+ cells in spleen or bone marrow, whereas both groups of irradiated recipients had normal numbers between 4 and 6 wk post-reconstitution. Normal levels of cytotoxic T cell activity by 8 wk after reconstitution were observed only in the irradiated C.B-17 and irradiated scid recipients. Analysis of mice reconstituted with cells from LTBMC indicates that these cultures contain lymphoid stem cells with significant proliferative and self-renewal potential, and that full reconstitution of lymphoid function requires prior irradiation of the scid recipient.     

Kinetics of the basic sections of the hemopoietic system in radiation chimeras]

During first 3 days after mice irradiation and syngeneic bone marrow transplantation in them the number of CFUs (about 0,5% of the injected cells) was stable, although the proliferation induction began 24 hours after transplantation. As it was shown by the method of "thymidine self-distruction". Twenty four hours later all the CFUs entered the mitotic cycle. On the contrary, the commited cells (granulopoesis precursors) compartment (CFUc) enters the logarithmic growth phase since the first day. The exponential growth of the CFUs number was observed from the 4th day simultaneously with the increasing of the proliferation rate of CFUc and the beginning of the recovery of the bone marrow cells total number. In late radiation chimeras (1 month after radiation and reconstitution) the total number of CFUs was 50--70% of the initial. The other hemopoetic parameters were in the normal limits.     

Prethymic T cell precursors express receptors for antigen

An anti-idiotype serum raised in BALB/c mice against syngeneic lymph node T cells from 2,4-dinitrofluorobenzene (DNFB)-sensitized mice was used to study the early expression of antigen receptors on developing T cells. Normal BALB/c bone marrow cells were treated with either anti-Thy-1.2 plus complement or anti-Thy-1.2 and anti-idiotype plus complement before use in the reconstitution of lethally irradiated syngeneic mice. Five weeks after reconstitution, recipient mice were assayed for both contact sensitivity (CS) and in vitro proliferative responses to DNFB. Mice reconstituted with bone marrow cells treated with both anti-Thy and anti-idiotype sera showed a significant decrease in reactivity to DNFB in both assay systems when compared with mice reconstituted with marrow treated with anti-Thy only. CS response to the noncross-reacting hapten oxazolone was identical in both recipient groups. Bone marrow mixing experiments showed no evidence of anti-idiotype-induced suppressor cells in these experiments. These data provide strong evidence that at least some T cell precursors express receptors for antigen prethymically.