ALA-PDT对多种白血病细胞破坏作用的实验研究

目的:本研究主要观察相同条件的5 氨基乙酰丙酸的光动力疗法(ALA PDT)对不同种类的白血病细胞株生存率的影响,以及细胞死亡类型的差异。方法:选择5种白血病细胞(K562、HL60、U937、MOLT 4和6T CEM)进行比较。用MTT法检测细胞的存活率,用AnnexinV FITC PI双染法检测细胞不同死亡类型的比例。结果:不同细胞对相同条件的ALA PDT的敏感程度不同,依次为U937相似文献   

5-氨基酮戊酸光动力疗法体外抑制断发毛癣菌肉芽肿株增殖研究

目的探讨5-氨基酮戊酸光动力疗法(5-Aminolevulinic acid photodynamic therapy,ALA-PDT)对体外培养的断发毛癣菌肉芽肿株的杀伤效应。方法将临床Majocchi肉芽肿患者皮损分离培养出的断发毛癣菌肉芽肿株,在马铃薯葡萄糖琼脂培养基上活化后制备菌悬液,与5mmol/L ALA共孵育后荧光显微镜观察原卟啉PpⅨ(ProtoporphyrinⅨ,PpⅨ)产生情况。实验分对照组、单药组、单光组和ALA-PDT组。对照组无处理。ALA-PDT组断发毛癣菌与5 mmol/L ALA共孵育6h后,采用功率密度为40mW/cm2的633nm红光以不同能量密度(50、100、150、175、200J/cm2)照射。单药组断发毛癣菌与5mmol/L ALA共孵育6h,不照光。单光组无ALA共孵育,只给予200J/cm2红光照射。通过数码相机拍摄照片及菌浓度评估ALA-PDT对断发毛癣菌肉芽肿株生长的抑制效应。结果荧光显微镜下可见明显砖红色荧光物质PpⅨ产生,当照光能量密度为175、200J/cm2时,照片显示菌落生长明显受限,数量减少,菌浓度计数分别为(0.53±0.058)×105 CFU/mL、(0.13±0.057)×105 CFU/mL,明显低于对照组、单药组、单光组及其他低能量密度ALA-PDT组(P0.05)。结论 ALA-PDT对断发毛癣菌肉芽肿株有明确的杀伤效应,可为临床ALA-PDT治疗皮肤癣菌感染提供理论依据。     

不同浓度5-氨基酮戊酸对光动力方法抗白念珠菌效果的影响

目的通过测定白念珠菌内不同光敏剂浓度下生成原卟啉IX(Pp IX)的水平及5-氨基酮戊酸光动力疗法(5-ALA-PDT)对白念珠菌的抑菌率,为临床选择最佳光敏剂浓度提供理论依据。方法制备白念珠菌悬液,与ALA避光孵育,采用激光共聚焦显微镜观察Pp IX产生情况,MTT法测定5-ALA-PDT对白念珠菌生长的抑制率。结果白念珠菌与ALA避光孵育后有荧光物质Pp IX产生,ALA光敏剂浓度与Pp IX强度呈正相关,当ALA浓度到达300 mg/m L时,Pp IX强度将不再增加。对照组无荧光物质出现。结论 ALA-PDT对白念珠菌抑制效应同光敏剂浓度密切相关。这为临床ALA-PDT治疗白念珠菌疾病提供了理论依据。     

5-氨基酮戊酸光动力疗法对不同疾病来源的耐甲氧西林金黄色葡萄球菌的体外杀伤作用

光动力疗法(photodynamic therapy,PDT)利用光敏剂与光源反应后产生的活性氧,破坏细菌组分,进而致细菌死亡。其多靶位杀伤特性在治疗耐甲氧西林金黄色葡萄球菌(methicillin-resistant Staphylococcus aureus,MRSA)感染方面有应用前景,但相关研究尚处于起步阶段。本研究MRSA菌株取自烧伤、急性咽炎、鼻窦炎和肺炎4类临床常见MRSA感染性疾病患者,使用5-氨基酮戊酸(5-aminolevulinic acid,ALA)光敏剂、发光二极管光源,于体外检测ALA介导的PDT(ALA-PDT)对MRSA菌株的杀伤作用。结果显示,经5mmol/L ALA孵育1h后,给予360J/cm~2强光[(633±10)nm]照射1h,ALA-PDT对MRSA菌株具有1.80log_(10)cfu的有效杀伤作用。结果提示,在相同实验条件和参数下,ALA-PDT对上述4种疾病来源的MRSA菌株体外杀伤作用无统计学差异。     

贝伐单抗对ALA—PDT诱导的新生血管形成和胶质瘤生长的影响

探讨贝伐单抗对低剂量5-氨基乙酰丙酸（5-Aminolevulinicacid,ALA）介导的光动力学疗法（photodynamic therapy,PDT）诱导的脑组织新生血管形成和U87脑胶质瘤生长的影响。通过将裸小鼠随机分为对照组、ALA．PDT预处置组（ALA：2．3×10-3mol／kg,能量密度：10J／cm2）、贝伐单抗预处置组（1．6×10-5mol／kg）和联合预处置组（ALA—PDT＋贝伐单抗）,并接受相应处置。第10d,检测PDT照射及相应区域内新生血管形成和VEGF表达并种植U87脑胶质瘤细胞,21d后观察肿瘤体积。与对照组比较,低剂量ALA-PDT预处置后新生血管增多、VEGF表达增高,肿瘤体积增大,这些变化在联合预处置组被抑制;贝伐单抗预处置组的血管形态和VEGF表达虽无明显变化,但肿瘤体积减小。研究结果表明低剂量ALA-PDT可通过刺激VEGF表达诱导照射区新生血管形成,这种微环境的改变有利于U87胶质瘤细胞生长,但这些作用可被贝伐单抗所抑制。     

脉冲磁场对白血病细胞HL60/ADR多药耐药的逆转效果及分子机制研究

目的:探讨脉冲磁场(pulsedmagnetic fields,PMF)对白血病细胞HL60/ADR多药耐药的逆转效果及其可能的分子机制.方法:生长曲线法检测PMF的细胞毒性;MTT法测定HL60、HL60/ADR的IC50及经不同参数PMF作用后HL60/ADR的IC50,计算耐药倍数和逆转倍数;流式细胞术检测PMF作用前后HL60/ADR细胞内药物蓄积变化及多药耐药相关蛋白(Multidrug Rcsistance Related Protcinl MRPI)阳性表达率的变化;RT-PCR法检测MRPI基因表达的变化.结果:单独PMF对HL60/ADR细胞的生长没有明显抑制作用,不同参数(频率为150Hz和250Hz,场强均为40mT,照射时间30min和1 h)的PMF均能有效逆转HL60/ADR的多药耐药,150 Hz/1 h作用最为明显,逆转倍数为5.891倍.PMF作用后Rh123在HL60/ADR细胞内的蓄积增加了近8.0%,而MRPl基因表达下调了68.3%,蛋白阳性表达率下调23.6%.结论:PMF能够通过下调MRPl基因和蛋白的表达.进而增加Rh123在细胞内的蓄积,功能性部分逆转白血病细胞的多药耐药.     

髓性白血病细胞HL60自发超微弱生物光子辐射研究

采用光子计数成像采集系统（PIAS）对髓性白血病细胞HL60自发的超微弱生物光子辐射进行了初步研究,获得了HL60细胞的生物光子强度与培养时间及细胞密度的关系。研究表明,HL60细胞的生物光子强度反映了细胞繁殖规律性及新陈代谢状况。为进一步探索肿瘤细胞与抗癌药物作用的生物光子效应,我们把TNF－β（肿瘤坏死因子）对悬浮HL60细胞进行处理,发现比同性质无TNF－β药物的对照组有更强的的超微弱光子辐射。     

急性早幼粒白血病HL60细胞电转染条件的优化

目的：比较不同电转染条件下,真核表达载体转染HL60细胞的效率,筛选得到针对HL60细胞最佳的电转染条件。方法：采用pDsRED-C1真核表达载体,分别在2mm和4mm电转杯中依照不同电转条件对HL60细胞进行转染,根据存活细胞所占比例确定电转参数;在转染48h后,比较不同质粒加入量及二甲基亚砜（dimethyl sulfoxide,DMSO）加入电转体系前后的细胞转染阳性率。调整G418筛选浓度,在选定转染条件下进行HL60细胞电转,采用流式细胞技术,细胞化学染色及超微结构观察,分析电转前后HL60细胞的生物学性状。应用相同条件再转染eYFP-C1质粒于HL60细胞,G418筛选后观察荧光表达情况。结果：HL60细胞在2mm和4mm电转杯中的死亡数量随电击强度和脉冲次数的增加而升高,且方形波较回旋波有更强的击穿细胞膜的能力;固定电转参数下,2mm和4mm电转杯中的HL60细胞电转阳性细胞数随加入质粒量的增加呈先升高后下降的趋势,且在相同质粒加入量,2mm电转杯比4mm电转杯有更高的转染效率;在相同电转参数和相同电转杯中,预冷条件下加入DMSO电转时阳性率比不加入DMSO进行电转的阳性率高近13倍;400μg/ml G418是最佳筛选浓度;选定最佳电转条件进行电转,通过筛选,没有发现细胞表面分化抗原CD11b和CD14的表达,细胞形态原始,未见凋亡现象发生。相同条件电转eYFP-C1空载质粒于HL60细胞仍然可以获得很好的转染效果。结论：HL60细胞电转染条件的改良,可以有效提高HL60细胞的电转阳性率,为后续细胞真核表达载体的转染及基因功能研究奠定基础。     

5-氨基γ-酮戊酸及其己酯衍生物对几种细胞株的光动力作用

5 氨基γ 酮戊 (ALA)及其己酯 (He ALA)具有内源生成光敏剂的特点 ,在肿瘤光动力探测及治疗中显示出了优势。ALA及He ALA对神经母细胞瘤、肝癌细胞及成纤维细胞的光动力作用被研究比较。由特征荧光光谱证实 ,经ALA或He ALA培养后 ,三种细胞内均可生成原卟啉 (PpIX)产物。激光扫描荧光显微镜显示 ,在经ALA或He ALA培养后的神经母细胞瘤中 ,PpIX均以弥散方式分布在细胞质中。PpIX在三种细胞中的积聚动力学过程不同 ,随着ALA或He ALA培育时间的增长 ,PpIX在肝癌细胞及成纤维原细胞中的积累增加 ,而在神经母细胞瘤中PpIX在 8h后已达到饱和。此外 ,在同样的培育条件下 ,神经母细胞瘤中PpIX的生成浓度明显高于肝癌细胞及成纤维细胞。经ALA培养及光照射后 ,可使近 90 %的神经母细胞瘤失活 ;而在同样条件下却只能杀伤 5 0 %左右的肝癌细胞及成纤维细胞。揭示了神经母细胞瘤对ALA光动力作用有极高的敏感性 ,并适于光动力治疗。与ALA相比 ,He ALA可在三种细胞内造成与ALA相近的杀伤率 ,但所用的药物浓度却比ALA低 10倍 ,显示He ALA具有极高的光动力灭活效率。因此在内源光动力治疗中 ,He ALA是一种极具开发前景的新药物。     

α-亚麻酸对高脂模型大鼠组织脂肪酸代谢的影响

研究不同ALA含量油脂对高脂模型大鼠组织脂肪酸代谢的影响.60只雄性Wistar大鼠分为正常组、高脂组、花生油组、13％、27％和55％ ALA含量油脂组,除正常组和高脂组外,其余各组在饲喂高脂饲料的同时采用灌胃方式连续给予2 mL/kg.bw剂量的受试油.试验6周后分别测定大鼠各组织脂肪酸组成.结果表明,高脂饮食能够降低大鼠各组织n-3脂肪酸含量,但摄入不同ALA油脂可显著增加组织n-3脂肪酸含量,并具有一定的剂量效应关系;但ALA及其代谢产物EPA、DPA和DHA的累积具有组织特异性,其中肾和心组织中ALA累积高于血浆、脑及肝组织,肝和脑组织中EPA和DPA含量增加较显著,而肾和心组织中EPA含量不变,各组织DHA含量增加不显著.不同ALA油脂组C18:3(n-6)和C20:3 (n-6)差异不显著,但与花生油组相比,其血浆、脑和肾组织C20:4含量显著降低.因此,富含ALA含量的油脂能够增加组织中ALA及其代谢产物在组织中的含量,提高其在脑组织中的分布比例,这可能是ALA具有心血管保护作用和促进脑生长发育的作用机制之一.     

Identification of molecular targets for selective elimination of TRAIL‐resistant leukemia cells. From spots to in vitro assays using TOP15 charts

The resistance of malignant cells to chemotherapy calls for the development of novel anti‐cancer drugs. TNF‐related apoptosis‐inducing ligand (TRAIL) is a pro‐apoptotic cytokine, which selectively induces apoptosis in malignant cells. We derived two TRAIL‐resistant HL‐60 subclones, HL‐60/P1 and HL‐60/P2, from a TRAIL‐sensitive HL‐60 acute promyelocytic leukemia cell line. To identify therapeutically exploitable “weaknesses” of the TRAIL‐resistant leukemia cells that could be used as molecular targets for their elimination, we performed proteomic (2‐DE) analysis and compared both TRAIL‐resistant subclones with the original TRAIL‐sensitive HL‐60 cells. We identified over 40 differentially expressed proteins. To significantly narrow the lists of candidate proteins, we excluded proteins that are known to be often differentially expressed, regardless of experiment type and tissue (the so‐called “TOP15” proteins). Decreased expression of DNA replication and maintenance proteins MCM7 and RPA32 in HL‐60/P1 cells, and the marked down‐regulation of enzyme adenosine deaminase in HL‐60/P2 cells, suggests increased sensitivity of these cells to DNA‐interfering drugs, and adenosine and its homologues, respectively. In a series of in vitro assays, we confirmed the increased toxicity of etoposide and cisplatin to TRAIL resistant HL‐60/P1 cells, and adenosine and vidarabine to HL‐60/P2, compared with TRAIL‐sensitive HL‐60 cells.     

HL-60细胞内DNA甲基化作用与RNA聚合酶活力的关系

以 S-腺苷酰 - L-甲硫氨酸 ( SAM)为诱导物 ,在 1 0 μmol/L最佳浓度下可诱导 HL- 60细胞分化达 1 6%左右 .HPLC测定结果证明 ,诱导物处理后 HL- 60细胞 DNA甲基化水平升高 .通过 3 H-UTP同位素参入法 ,测定了不同处理时间和不同浓度 SAM对 HL- 60细胞 DNA模板体外转录活性的影响 ,发现体外活力下降 .比较了不同浓度α-鹅膏蕈碱存在下 RNA聚合酶活力的变化 ,结果表明 SAM处理后细胞中不同 RNA转录产物所占份额改变     

重组人粒系集落刺激因子(rhG-CSF)对白血病细胞HL-60生长的影响

本文研究了rhG CSF对人白血病细胞系HL 6 0的作用。结果表明 :rhG CSF能够显著抑制HL 6 0细胞生长和C myc基因的表达 ,降低3H TdR的摄入。在含rhG CSF的培养液中经过 2～ 5天的培养 ,部分HL 6 0细胞具备NBT还原能力。这或许说明rhG CSF能导致HL 6 0细胞向成熟方向分化的结果。     

Proanthocyanidins from Barley Bran Potentiate Retinoic Acid-induced Granulocytic and Sodium Butyrate-induced Monocytic Differentiation of HL60 Cells

Polyphenol extract from barley bran (BPE) induced nitro blue tetrazolium (NBT) reducing activity and alpha-naphthyl butyrate esterase activity in HL60 human myeloid leukemia cells. Because BPE induced the biochemical markers of HL60 cell differentiation, we investigated the effects of proanthocyanidins isolated from BPE on the HL60 cell differentiation of HL60 cells. Prodelphinidin B-3, T1, T2, and T3 induced 26-40% NBT-positive cells and 22-32% alpha-naphthyl butyrate esterase-positive cells. Proanthocyanidins potentiated retinoic acid (all-trans-retinoic acid)-induced granulocytic and sodium butyrate-induced monocytic differentiation in HL60 cells.     

Inhibition of the MAPK pathway abrogates BCL2-mediated survival of leukemia cells after exposure to low-dose ionizing radiation.

The ability of low-dose ionizing radiation (1 Gy) to modulate the activities of the mitogen-activated protein kinase (MAPK) and Jun NH2-terminal kinase (JNK1) cascades in human myeloid leukemia (HL60/pCEP4) cells and in cells overexpressing the anti-apoptosis protein BCL2 (HL60/Bcl-2) was investigated. Radiation exposure caused prolonged (3-4 h) activation of MAPK in HL60 cells. The ability of radiation to activate the MAPK pathway was attenuated by 30% in cells overexpressing BCL2. In contrast, low-dose irradiation of HL60/pCEP4 and HL60/Bcl-2 cells failed to modulate JNK1 activity. Inhibition of the MAPK pathway by use of the specific MEK1/2 inhibitor (10 microM PD98059) in both HL60/pCEP4 and HL60/Bcl-2 cells prior to irradiation permitted a similar prolonged radiation-induced activation of JNK1. Furthermore, combined treatment with PD98059 and radiation in both cell types caused a large decrease in growth of cells in suspension culture, a large increase in apoptosis, and a 90% decline in clonogenicity when compared to either treatment alone. Reduced proliferation after combined irradiation and PD98059 treatment in both cell types correlated with reduced Cdc2 activity and arrest in G2/M phase of the cell cycle. These data demonstrate that inhibition of MEK1/2 leading to blockade of the MAPK activation increases the radiation sensitivity of HL60 cells and decreases the ability of these cells to recover from the radiation-induced arrest at the G2/M-phase cell cycle checkpoint. In addition, our data demonstrate that elevated expression of BCL2 does not abrogate the ability of inhibition of MAPK to potentiate radiation-induced cell death in HL60 cells.     

Defective chemiluminescence response in differentiated HL60 cells due to impaired degranulation

In the presence of dimethyl sulfoxide, the promyelocytic leukemic cell line, HL60, differentiates into apparently mature polymorphonuclear leukocytes. When correlating the superoxide production from HL60 cells with the number of phagocytozing and NBT-positive cells, no difference was observed in comparison with normal peripheral blood leukocytes. In contrast, the luminol-dependent chemiluminescence was greatly impaired in the differentiated HL60 cells. Analysis of degranulation, i.e., release of myeloperoxidase and N-acetyl-beta-glucosaminidase- and myeloperoxidase-mediated iodination by HL60 cells, suggested that the defective chemiluminescence response observed in HL60 cells may be due to impaired release of myeloperoxidase from azurophilic granulae. This may lead to impaired microbicidal activity in these cells.     

S-腺苷酰L-甲硫氨酸 (SAM)对 HL-60细胞 DNA甲基化酶活力和甲基化水平的影响(英文)

 以 S-腺苷酰 - L-甲硫氨酸 (SAM)为诱导物 ,在 1 0 μmol/L最佳浓度下造成 1 6%的 HL- 60细胞分化 .HPLC检测结果表明 ,细胞基因组 DNA甲基化水平升高 .通过3H甲基同位素参入法研究细胞 DNA甲基化酶活力 ,则发现在细胞分化过程中酶活力未见升高 .说明细胞基因组甲基化水平升高并不是胞内 DNA甲基化酶催化能力改变的结果 ,而是由于 SAM进入细胞提供过量甲基造成的 .     

Notch signaling maintains proliferation and survival of the HL60 human promyelocytic leukemia cell line and promotes the phosphorylation of the Rb protein

The Notch signaling pathway has been implicated in the development of several leukemia and lymphoma. In order to investigate the relationship between Notch signaling and acute myeloid leukemia (AML), in this study, we expressed a recombinant Notch ligand protein, the DSL domain of the human Jagged1 fused with GST (GST-Jag1). GST-Jag1 could activate Notch signaling in the human promyelocytic leukemia cell line HL60, as shown by a reporter assay and the induced expression of Notch effector gene Hes1 and Hes5. However, GST-Jag1 had no effect on the proliferation and survival of HL60 cells. HL60 cells expressed both Notch ligands and receptors, and had a potential of reciprocal stimulation of Notch signaling between cells. We, therefore, blocked Notch signaling in cultured HL60 cells using a γ-secretase inhibitor (GSI). We found that GSI inhibited the proliferation of HL60 cells significantly by blocking the cell-cycle progression in the G1 phase. Furthermore, GSI induced remarkably apoptosis of HL60 cells. These changes in GSI-treated HL60 cells correlated with the down-regulation of c-Myc and Bcl2, and the low phosphorylation of the Rb protein. These results suggested that reciprocal Notch signaling might be necessary for the proliferation and survival of AML cells, possibly through the maintenance of the expression of c-Myc and Bcl2, as well as the phosphorylation of the Rb protein.     

Interaction of Actinobacillus actinomycetemcomitans outer membrane vesicles with HL60 cells does not require leukotoxin

Outer membrane derived vesicles (MVs) secreted by Actinobacillus actinomycetemcomitans JP2 contain a membranolytic leukotoxin and are toxic to human HL60 cells. To determine how MVs interact with human target cells, HL60 cells were incubated with vesicles, reacted with anti-vesicle antibodies and a FITC-labelled reporter, and visualized by confocal scanning laser microscopy. Target cells rapidly became reactive with anti-vesicle antibodies upon exposure to vesicles. Confocal microscopy showed that labelling occurred primarily in the cytoplasmic membrane and that very little internal fluorescence was observed. The cytoplasmic membrane of HL60 cells was also strongly labelled after exposure to MVs that contained the fluorescent phospholipid, SP-DiOC18. In contrast, incubation of cells with free SP-DiOC18 resulted primarily in the labelling of internal structures of HL60 cells. These results suggest that A. actinomycetemcomitans MVs associate with, or are incorporated into the cytoplasmic membrane of HL60 cells. The leukotoxin is a membranolytic cytotoxin and cells exposed to MVs were lysed by vesicle-associated toxin in a time and dose-dependent manner. However, cells became reactive with anti-vesicle antibodies when MVs were added in the presence of inhibitors of leukotoxin-mediated lysis or when sublytic doses of MVs were analysed. In addition, MVs produced by an isogenic leukotoxin-deficient strain of A. actinomycetemcomitans JP2 were non-toxic but rapidly interacted with HL60 cells. These results suggest that A. actinomycetemcomitans MVs can deliver leukotoxin to HL60 cells but that the association of vesicles with the cytoplasmic membrane occurs independently of the leukotoxin polypeptide.