小剂量16O8+离子预辐射减轻大剂量辐射所致小鼠睾丸组织损伤

为了了解小剂量重离子辐射诱导小鼠睾丸结构的适应性反应,采用小剂量(0.05Gy)~(16)O~(8 )离子照射B6C3F_1雄性小鼠睾丸。4h后,再给予2Gy~(16)O~(8 )离子照射。照射后第35天取材在光镜下观察睾丸结构。结果显示,大剂量(2Gy)照射明显损伤睾丸组织,主要表现为曲精细管直径几乎减小一半,精管内各发育阶段的生殖细胞减少或消失,特别是精原细胞几乎完全消失。而Leydig细胞和Sertoli细胞仅有轻度核固缩及胞浆减少。提示睾丸生殖细胞的辐射敏感性明显高于其间质组织细胞。预先给予小剂量(0.05Gy)照射可明显减轻随后大剂量(2Gy)辐射对睾丸组织的损伤。提示小剂量重离子辐射可诱导小鼠睾丸结构明显的适应性反应。     

TCTP在辐射诱导胶质瘤细胞旁效应中的作用及机制研究

目的:研究肿瘤翻译控制蛋白(TCTP)在辐射诱导胶质瘤细胞旁效应中的作用及机制。方法:给予不同剂量的X射线照射U87、SHG44两种胶质瘤细胞,观察U87以及SHG44细胞的克隆形成率,并在给予最佳照射剂量后,通过Western Blot检测TCTP蛋白表达水平。将经过最佳X射线照射剂量的U87以及SHG44两种胶质瘤细胞与未经过辐射照射的细胞放在一起共培养,通过MTT实验检测胶质瘤细胞的增殖率,Western Blot检测共培养的胶质瘤细胞与经过辐射的胶质瘤细胞中Caspase3蛋白表达水平。结果:U87以及SHG44两种胶质瘤细胞的克隆形成率随着X射线照射剂量增加而显著性降低(P0.05),给予最佳X射线照射剂量后,与未经过X射辐射照射后的细胞相比,其TCTP蛋白表达水平明显升高(P0.05)。经过辐射照射与未经过辐射照射的胶质瘤细胞经过共培养后,与经过辐射的胶质瘤细胞相比,细胞的增殖率明显升高,同时共培养的胶质瘤细胞与经过辐射的胶质瘤细胞相比,Caspase3的蛋白表达明显降低(P0.05)。结论:TCTP的表达增高能够诱导未经过辐射的U87以及SHG44两种胶质瘤细胞的抗凋亡作用增强,其作用机制可能与Caspase3的表达降低有关。     

电离辐射对伤口巨噬细胞生长因子基因表达的影响及苯妥因钠的作用

研究了电离辐射全身和局部照射对伤口巨噬细胞(MΦ)生长因子基因表达的影响及苯妥因钠的作用。伤口MΦ从置入大鼠背部的聚乙烯醇海绵中收集,用原位杂交技术测定血小板源性生长因子-B(PDGF-B)和转化生长因子-β(TGF-β_1)mRNA在MΦ表达的阳性细胞率。结果表明,6Gy全身辐射后伤口MΦ PDGF-B和TGF-β_1 mRNA阳性表达率明显下降,20Gy局部辐射后无明显影响;苯妥因钠对正常伤口、全身辐射和局部辐射后的伤口MΦ PDGF-B和TGF-β_1 mRNA表达的阳性率都有明显的提高。这说明伤口MΦ生长因子基因表达的降低与全身辐射后创伤愈合延迟有关;苯妥因钠明显增加伤口MΦ生长因子基因表达而有利于创伤愈合。     

810nm弱激光照射对大鼠急性脊髓损伤后巨噬细胞极化的作用研究

本研究构建急性大鼠脊髓夹伤模型,并将大鼠随机分为单纯脊髓损伤对照组及脊髓损伤联合弱激光照射组。照射组应用810 nm波长,150 m W照射功率,照射光斑0.3 cm^2的弱激光对脊髓损伤区进行经皮照射,连续照射3天,7天或14天。应用免疫荧光、免疫印迹实验方法,测定脊髓损伤区巨噬细胞及小胶质细胞的极化表达。应用酶联免疫吸附法测定脊髓损伤区白细胞介素4的表达情况。应用坚牢蓝髓鞘染色测定两组损伤脊髓中髓鞘保留的差异。采用BBB评分对两组大鼠后肢运动功能的恢复进行评估。结果表明,810 nm弱激光对脊髓损伤区连续照射3天,7天后,可显著减少M1型巨噬细胞及其标志物诱导型一氧化氮合酶的表达,在7天时间增加M2型巨噬细胞及其标志物精氨酸酶1的表达。弱激光照射组白细胞介素4的表达明显增加。损伤后14天,弱激光照射组脊髓损伤区髓鞘保留面积比值明显提高。损伤后7天及14天时,弱激光照射组大鼠的BBB评分明显升高。该实验结果表明,810 nm弱激光经皮照射,可增加大鼠急性脊髓损伤区M2型巨噬细胞及小胶质细胞的表达,并减少脊髓损伤后的髓鞘脱失,促进脊髓损伤大鼠运动功能的恢复。     

γ射线长期低剂量照射对猕猴淋巴细胞染色体的效应

在急性辐射情况下,外周血淋巴细胞染色体畸变是生物剂量测定中最容易定量的方法。但小剂量慢性照射下染色体损伤的近、远期效应尚不清楚。我们曾用γ射线对猕猴及大白鼠低剂量(分别为2.55rad/天和10rad/天)长期照射观察外周血淋巴细胞染色体效应,在这个研究工作基础上,我们又选用更低的剂量率(0.8rad/天)进一步探讨小剂量慢性照射对猕猴外周血淋巴细胞染色体的效应,以便提供小剂量慢性照射对人类的损伤恢复规律的资料。     

TAB182对电离辐射诱发细胞周期G2/M阻滞的调节作用

TAB182是一个端锚聚合酶1（tankyrase 1）结合蛋白,它在体外能够被tankyrase 1发生二磷酸腺苷核糖基化(PAR)修饰,其生物学功能目前尚不明确.本研究发现,TAB182蛋白水平受电离辐射诱导表达,HeLa细胞经过4 Gy照射处理时,TAB182在2 h表达含量最高; 经过不同剂量照射处理,2 h后2 Gy、4 Gy照射剂量组HeLa细胞中TAB182的表达有明显增加. 通过shRNA沉默HeLa细胞中TAB182基因表达,导致其对4 Gy及以下剂量 辐射的敏感性增加,但对8 Gy大剂量照射的敏感性没有明显变化. 与对照组相比,4 Gy照射诱发TAB182基因沉默细胞的G2/M期阻滞时间显著延长.抑制TAB182表达导致细胞中DNA损伤反应蛋白DNA PKcs、ATM、Chk2的表达水平显著降低. 实验结果提示,TAB182蛋白参与放射DNA损伤信号反应和调控细胞周期G₂/M进程.     

某些抗氧化剂对体外辐射诱导的红细胞钾离子渗漏的影响

脂质体辐射研究说明钾离子的渗漏量是照射剂量的函数,并与脂质过氧化物的生成相平行。Kocmierska Grodzka 对全身照射大鼠肝体外灌注试验观察到灌注液中钾离子含量增加,并与肝溶酶体脂质过氧化物含量升高相关。Prince等对缺乏和不缺乏维生素E(VE)小鼠的红细胞(RBC)体外辐射研究发现,前者钾离子的渗漏远较后者为明显。以上事实说明,辐射诱导的RBC钾离子渗漏与RBC膜的脂质过氧化作用有关。辐射脂质过氧化作用的特点之一是剂量率效应。最近Konings报道了辐     

小剂量~(60)Coγ线长期照射对猕猴睾丸组织的影响

前言我们先前的工作已证实,睾丸在小剂量γ线长期照射下极为敏感;辐射的损伤效应比其他器官出现早,且较严重;生精过程受到严重扰乱,各级生精细胞急骤减少,精小管退化萎缩,最终导致绝精,完全丧失生殖能力。本文试图介绍进一步研究在小剂量射线长期照射下睾丸组织的损伤特点,探讨其损伤与每日剂量及总累积剂量的关系,进而对使猕猴     

高能电子束超剂量照射与效应关系的探讨——人周血淋巴细胞核损伤指标的比较观察

为了探讨在大剂量辐射条件下建立生物量计的可能,本实验研究了在10MeV电子束照射后,人体外周血淋巴细胞各种核损伤指标的改变与剂量(0—40Gy)间的关系,结果表明,随着照射剂量的增大,复合核损伤指标——核异常率、微核率、核固缩率和核裂解率亦随之上升,在0—20Gy范围内,与剂量呈线性关系,相关系数显著性检验P<0.01的核损伤指标是:核异常率、微核率。P<0.05的是核变形率;在0—40Gy范围内,与之呈线性关系,P<0.01的仅有核固缩率。和染色体畸变分析相比,核异常检测方法简便,可反映超剂鞋(如>10Gy)辐射的损伤,值得引起研究者的注意。     

JNK通路对M2巨噬细胞极化及其肿瘤效应的影响

探究了JNK通路对M2巨噬细胞极化及M2介导的促肿瘤效应的影响。构建单核细胞THP1来源M2 巨噬细胞模型(THP1-M2),将细胞分为3组: 用PMA 诱导的未活化巨噬细胞组(M0),用PMA、IL-4处理及阴性干扰(DMSO)的M2型巨噬细胞组(M2),用特异性抑制剂阻断JNK通路的M2 型巨噬细胞组(M2-JNKI)。实时荧光定量PCR检测M2 表型marker基因的表达;免疫蛋白印迹法检测M2 表型marker蛋白水平;细胞划痕试验检测巨噬细胞迁移能力;流式细胞数检测786O及OSRC2凋亡。结果与THP1-M2组相比,阻断JNK通路的M2组M2表型marker表达明显下降,同时其细胞迁移能力也呈下降趋势。且阻断JNK通路后,M2巨噬细胞抑制肾癌细胞凋亡的能力减弱。结果表明,抑制JNK通路后,M2巨噬细胞极化状态受损,其促肿瘤效应可转变为抗肿瘤效应。     

Radiation effects on expression of FC-receptor of alveolar macrophages of rat and their specific phagocytosis

BCG-activated alveolar macrophages (AM) of Wistar rats were irradiated with different doses of gamma-ray in vitro. The effects of radiation on the expression of their Fc-receptor and specific phagocytic activity were observed. AM, after irradiation with doses of 0, 100, 300 and 500 Gy, showed decreasing phagocytic activity to chicken red blood cells (CRBC) opsonized with anti-CRBC antibody with no change in phagocytic indices. The expression of Fc-receptor of AM was, however, increased.     

Impaired functional activity of alveolar macrophages from GM-CSF-deficient mice

We hypothesized that pulmonary granulocyte-macrophage colony-stimulating factor (GM-CSF) is critically involved in determining the functional capabilities of alveolar macrophages (AM) for host defense. To test this hypothesis, cells were collected by lung lavage from GM-CSF mutant mice [GM(-/-)] and C57BL/6 wild-type mice. GM(-/-) mice yielded almost 4-fold more AM than wild-type mice. The percentage of cells positive for the beta(2)-integrins CD11a and CD11c was reduced significantly in GM(-/-) AM compared with wild-type cells, whereas expression of CD11b was similar in the two groups. The phagocytic activity of GM(-/-) AM for FITC-labeled microspheres was impaired significantly compared with that of wild-type AM both in vitro and in vivo (after intratracheal inoculation with FITC-labeled beads). Stimulated secretion of tumor necrosis factor-alpha (TNF-alpha) and leukotrienes by AM from the GM(-/-) mice was greatly reduced compared with wild-type AM, whereas secretion of monocyte chemoattractant protein-1 was increased. Transgenic expression of GM-CSF exclusively in the lungs of GM(-/-) mice resulted in AM with normal or supranormal expression of CD11a and CD11c, phagocytic activity, and TNF-alpha secretion. Thus, in the absence of GM-CSF, AM functional capabilities for host defense were significantly impaired but were restored by lung-specific expression of GM-CSF.     

Characteristics of the membranes and functional activity of phagocytic alveolar macrophages

Alveolar macrophages (AM) accumulate products of lipid peroxidation (PLP) in the time of phagocytosis of zymosan particles (ZP) during 4 hours, that lead to increase of lipid viscosity and decrease surface membrane area, which were studied by fluorescent probes pyrene and HSPH-14. Preliminary stimulation of AM by i/v ZP-injection of A(100 mg/kg before 5 days) lead to a decrease of lipid membrane viscosity and intensification of AM functional activity. During phagocytosis of ZP experimental cells accumulate much less PLP, than control cells, and promote support of viscosity on a more low level, and functional activity (phagocytic, adhesion properties)--on more high level, than in control cells.     

ICAM-1 facilitates alveolar macrophage phagocytic activity through effects on migration over the AEC surface

We postulate that intercellular adhesion molecule-1 (ICAM-1) on type I alveolar epithelial cells (AEC) facilitates phagocytic activity of alveolar macrophages (AM) in the alveolus. When wild-type and ICAM-1-deficient mice were inoculated intratracheally with FITC-labeled microspheres, AM phagocytosis of beads (after 1 and 4 h) was significantly reduced in ICAM-1-/- mice compared with controls. To focus on ICAM-1-mediated interactions specifically involving AM and AEC, rat AM were placed in culture with rat AEC treated with neutralizing anti-ICAM-1 F(ab')(2) fragments. Blocking ICAM-1 significantly decreased the AM phagocytosis of beads. Planar chemotaxis of AM over the surface of AEC was also significantly impaired by neutralization of AEC ICAM-1. ICAM-1 in rat AEC is associated with the actin cytoskeleton. Planar chemotaxis of AM was also significantly reduced by pretreatment of the AEC monolayer with cytochalasin B to disrupt the actin cytoskeleton. These studies indicate that ICAM-1 on the AEC surface promotes mobility of AM in the alveolus and is critically important for the efficient phagocytosis of particulates by AM.     

An innate immune system cell is a major determinant of species-related susceptibility differences to fungal pneumonia

Rats and mice are considered resistant and susceptible hosts, respectively, for experimental cryptococcosis. For both species, alveolar macrophages (AM) are central components of the host response to pulmonary Cryptococcus neoformans infection. We explored the role of AM in three strains of mice and three strains of rats during cryptococcal infection by comparing the outcome of infection after macrophage depletion using liposomal clodronate. AM depletion was associated with enhancement and amelioration of disease in rats and mice, respectively, as measured by lung fungal burden. The apparent protective role for AM in rats correlated with enhanced anti-cryptococcal activity as measured by phagocytic activity, oxidative burst, lysozyme secretion, and ability to limit intracellular growth of C. neoformans. Furthermore, rat AM were more resistant to lysis in association with intracellular infection. In summary, differences in AM function in rats and mice suggest an explanation for the species differences in susceptibility to C. neoformans based on the inherent efficacy of a central effector cell of the innate immune system.     

Morphological heterogeneity and functional status of the alveolar macrophages from bronchoalveolar lavage during the development of tuberculous inflammation in guinea pigs

Alveolar macrophages (AM) isolated from bronchoalveolar lavage of guinea pigs obtained in the course of generalized tuberculosis development was studied by electron microscopy. The protein content, activity of cathepsins B and D, as well as macrophage and neutrophil elastase activity have been determined. It was shown that during the first month of specific process development an influx of young biosynthesizing AM building up the lysosomal apparatus was observed; phagocytic, digesting and secretory functions of mature cells were enhanced. Progressing of tuberculosis was accompanied by the inhibition of biosynthetic processes in AM, a decrease in digesting and secretory functions, which were manifested at the biochemical and then at the electron microscopic levels and were of a prognostic value.     

异质性荧光染色的巨噬细胞功能研究I．异质性荧光染色的巨噬细胞吞噬活性

利用淀粉多糖和免疫促进剂（白喉类毒素和卡介苗）诱导和活化小鼠腹腔巨噬细胞,观察了四种异质性荧光染色的巨噬细胞非特异性和特异性吞噬活性。实验证明,深蓝色和淡蓝色荧光的巨噬细胞是分化程度低的幼稚细胞,非特异性吞噬功能较弱,但在特异性吞噬过程中呈现了活跃的吞噬活性,特别是在免疫促进剂的活化下,它们的特异性吞噬功能显著增强、淡蓝绿色荧光的巨噬细胞是分化程度较高、非特异性和特异性吞噬功能最旺盛的巨噬细胞,而黄色荧光的巨噬细胞是分化程度最高、特异性吞噬功能较减退的巨噬细胞。     

Mycobacterium tuberculosis resides in nonacidified vacuoles in endocytically competent alveolar macrophages from patients with tuberculosis and HIV infection

Alveolar macrophages (AM) are the first professional phagocytes encountered by aerosols containing infections in the lungs, and their phagocytic capacity may be affected by these infections or environmental particles. The aim of this study was to evaluate the innate endocytic and phagocytic properties of human AM obtained from patients with pulmonary tuberculosis and to characterize the vacuoles in which Mycobacterium tuberculosis bacilli reside in vivo. AM were obtained by bronchoalveolar lavage from patients with suspected tuberculosis and from asymptomatic volunteers (controls). Clinical case definitions were based on mycobacterial culture of respiratory specimens and HIV serology. To assess phagocytosis, endocytosis, and acidification of the endosomal system, AM were cultured with IgG-coated polystyrene beads, dextran, and a pH-sensitive reporter (3-(2,4-dinitroanilino)-3-amino-N-methyldipropylamine) and were evaluated by light and immunoelectron microscopy. Cells from 89 patients and 10 controls were studied. We found no significant difference between the two groups in the ability of AM either to ingest beads and dextran or to deliver them to acidified lysosomes. In AM from patients with tuberculosis, the bacilli were located in vacuoles that failed to accumulate endocytosed material and were not acidified. We concluded that AM from patients with tuberculosis and HIV infections were competent to endocytose and phagocytose material and to deliver the material to functional, acidified lysosomes. M. tuberculosis residing in these AM arrests the progression of their phagosomes, which fail to fuse with acidified lysosomes. This confirms, for the first time in humans with tuberculosis and HIV, the conclusions from previous animal and in vitro studies.     

Study of rat pulmonary macrophages as affected by hydrocortisone administration and adrenalectomy

The blood clearance rate of inert colloidal particles and the number of rat lung interstitial phagocytic cells decrease considerably on the 7th day after daily subcutaneous hydrocortisone acetate (HC) injection at a dose of 125 mg/kg. The number of cells in the bronchoalveolar lavage (BAL) increases more than 5-fold, and the absolute quantity of neutrophils is 66 times higher than in the control. Phagocytic and microbicidal activity of HC-treated animal alveolar macrophages (AM) decreases. Stimulation with zymosan led only to the recovery of the normal parameters of mononuclear phagocytosis system (MPC) and its pulmonary compartment activity. The parameters of MPS and AM studied increase on the 7th day after bilateral adrenalectomy (AE). The number of BAL cell increases 1.4-fold due to the animals' death immediately after intravenous zymosan injection because of total hemorrhage. The data obtained testify to the influence of glucocorticoids on the composition and activity of bronchoalveolar space cells, which in turn determine the resistance of the lung tissue.     

In vivo interaction between alveolar macrophages and Cryptococcus neoformans

In vivo interactions of rabbit alveolar macrophages (AM) and Cryptococcus neoformans, a yeast pathogenic for humans, were studied. As a control, inert silica particles of a similar diameter (5–6 μm) were used. Of 16 rabbits, 6 were instilled intratracheally with fluorescein-labelled heat-killed C. neoformans, 6 with fluorescein-labelled silica particles and 4 with saline only. After 24 h, the AM were collected by lung lavage, and phagocytosis, oxidative metabolism, phagolysosomal pH and morphology were studied. The accumulated number of yeasts attached to the AM was almost the same for C. neoformans as for the silica particles. The ingested fraction of C. neoformans was even higher than that of the silica particles. Quantitative NBT reduction by the AM, reflecting their oxidative metabolism, was markedly increased by exposure to C. neoformans for 24 h. The phagolysosomal pH was on the average lower in phagolysosomes with C. neoformans than with the silica particles, although approximately 2% of the phagolysosomes with C. neoformans had neutral pH. Phagolysosomes with neutral pH was not observed for silica particles. Electron microscopy showed presence of C. neoformans in phagolysosomes of AM. The conclusion of this study is that the phagocytic activity, oxidative metabolism and phagolysosomal pH AM against C. neoformans are significant 24 h after the exposure. This revised version was published online in June 2006 with corrections to the Cover Date.