弱激光对脂质体介导的血管平滑肌细胞基因转染的影响

本研究采用阳离子脂质体介导外源基因转染体外培养的兔血管平滑肌细胞（ＳＭＣ）,在基因转染过程中给予激光照射,用细胞化学染色方法测定基因转染阳性率。结果显示：用５１０．６ｎｍ激光于基因转染前,以功率密度１ｍｗ／ｃｍ２,能量密度２、４、６Ｊ／ｃｍ２和５ｍＷ／ｃｍ２,４、６Ｊ／ｃｍ２;及１０ｍＷ／ｃｍ２,２Ｊ／ｃｍ２进行照射均能显著提高基因转染率（ｐ＜０．０５）;于基因转染后即刻以功率密度１ｍＷ／ｃｍ２、能量密度２Ｊ／ｃｍ２和５ｍＷ／ｃｍ２、６Ｊ／ｃｍ２照射也能提高基因转染率（ｐ＜０．０５）。而用６２７．８ｎｍ激光照射对基因转染率无显著影响     

血啉甲醚体外光敏效应观察

本文用化学发光法检测ＨＭＭＥ的’Ｏ２和ＲＯＳ产量,并与ＨｐＤ相比较,同时观察ＨＭＭＥ光敏效应与浓度、激光照射功率密度、照射时间、激光波长的关系。结果显示：ＨＭＭＥ浓度在２．５－４０μｇ／ｍｌ范围内,其光敏效应随浓度的增加而呈线形上升,以后便略下降;５７８．２ｎｍ激光以１０ｍＷ／ｃｍ＾２照射２．５μｇ／ｍｌ,ＨＭＭＥ的’Ｏ２和ＲＯＳ产量是ＨｐＤ的８倍;ＨＭＭＥ光敏效应与激光照射的功率密度密切相关。各     

510.6nm激光照射对兔血管平滑肌细胞增殖的影响

本文用５１０．６ｎｍ 波长激光以功率密度１、５、１０ ｍ Ｗ／ｃｍ ２ 和能量密度２、４、６Ｊ／ｃｍ ２ 照射体外培养的兔血管平滑肌细胞（ＳＭＣ）,通过３Ｈ－ ＴｄＲ掺入率和细胞生长曲线测定细胞增殖率。结果显示,上述激光照射量均能抑制细胞增殖率,其中以１０ｍ Ｗ／ｃｍ ２ 组的作用最为显著     

CO2激光辐射奶山羊精液生物学效应的研究

本研究表明,３．５７Ｊ／ｃｍ＾２和７．４Ｊ／ｃｍ６２激光组可以改善精液品质,提高精子的代谢功能状态,以增强精子活力,认为是最佳剂量;１４．２８Ｊ／ｃｍ６２激光组虽然对精子的代谢,活力有效应,但不能维持,认为是临界剂量;２８．５６Ｊ／ｃｍ＾２激光对精子的损害作用,认为是抑制剂量。     

叠架极低频噪声磁场诘抗连接微波对水迷宫大鼠认知行为负作用的实验观察

暴露于２４５０ＭＨｚ连续（ＣＷ）微波（功率密度：２ｍＷ／ｃｍ＾２,ＳＡＲ：１．２Ｗ／ｋｇ）的大鼠在水迷宫训练期特别是检测期显示了认知功能的下降,表明了空间“工作记忆”的消弱。但是,同时施加一个极低频（ＥＬＥ）噪声磁场（ｒｍｓ：１０μＴ）,上述负效应完全消失。这一动物行为学结果暗示,时间不相干而空间相干的低强度ＥＬＦ噪声磁场能长程抗拮大鼠对连续微波的负作用。     

倍频Nd：YAG激光对钝项螺旋藻的诱变效应

利用倍频Ｎｄ：ＹＡＧ激光（波长５３２ｎｍ,功率５００ｍＷ,功率密度１６０ｍＷ／ｃｍ＾２）诱变钝项螺旋藻,辐照时间为１５ｍｉｎ、１０ｍｉｎ、５ｍｉｎ通过测定藻丝形态参数、叶绿素α、β－胡萝卜素、生长速度,比较倍频Ｎｄ：ＹＡＧ激光对钝项螺旋藻生长的影响。实验结果表明：与出发株相比,经倍频Ｎｄ：ＹＡＧ激光辐照后,藻丝形态发生变化,藻丝长、螺旋数、螺旋长变小;１５ｍｉｎ,１０ｍｉｎ辐照组出现螺旋变松驰;１     

剪切应力对毛细血管内皮细胞代谢的影响

建立的平行平板流动腔装置适用于研究血管内皮细胞代谢对剪切流场的响应。将培养的人胚肾小球血管单层内皮细胞置于剪应力分别为５×１０－５Ｎ／ｃｍ２,１×１０－４Ｎ／ｃｍ２和１．５×１０－４Ｎ／ｃｍ２的定常层流中剪切２５小时,样品中的内皮素分泌量用放射免疫法测定。结果表明,剪应力水平对内皮细胞内皮素的代谢活动有显著影响。与静态培养对照,低水平的剪应力（５×１０－５Ｎ／ｃｍ２、１×１０－４Ｎ／ｃｍ２）促进内皮素的分泌,而较高水平的剪应力（１．５×１０－４Ｎ／ｃｍ２）抑制内皮素的分泌;剪应力对内皮素累积含量的影响比之分泌速率更大     

水稻叶片磷酸烯醇式丙酮酸磷酸酯酶活性及其部分特性

从水稻（Ｏｒｙｚａ ｓａｔｉｖａ）叶片分离出对磷酸烯醇式丙酮酸（ＰＥＰ）较专一的ＰＥＰ磷酸酯酶,其Ｋｍ （ＰＥＰ）为０．４２ ｍ ｍ ｏｌ／Ｌ,作用ｐＨ范围较窄,最适ｐＨ ８．７。它在ｐＨ ６．２—９．５ 范围内及４０℃以下较稳定。Ｐｉ对酶活性影响不大,仅在大于５ ｍ ｍ ｏｌ／Ｌ时表现出轻微的抑制作用。Ｍｇ２＋ 对酶活性具激活作用,在Ｍｇ２＋ 存在条件下,ＣａＣｌ２、ＣｏＣｌ２、ＣｕＳＯ４、ＦｅＳＯ４ 和ＺｎＳＯ４ 均表现抑制作用     

兼性CAM植物NAD—苹果酸酶的行为研究

以土三七（Ｓｅｄｕｍ ａｉｚｏｏｎ）和露花（Ｍｅｓｅｍ ｂｒｙａｎｔｈｅｍ ｕｍ ｃｏｒｄｉｆｏｌｉｕｍ ）为材料,对兼性景天酸代谢（ＣＡＭ）植物的ＮＡＤ－苹果酸酶作了初步研究。当有５ ｍ ｍ ｏｌ／ＬＭｎＣｌ２、６ ｍ ｍ ｏｌ／ＬＭａｌ和５０ μｍ ｏｌ／ＬＣｏＡ 存在时,其最适ｐＨ 为７,且在低ｐＨ（７ 以下）范围内活性较高,而在高ｐＨ（７以上）范围内活性较低。该酶活性有季节性的变化,在７ 月份酶活性达最高峰,这与羧化系统的磷酸烯醇式丙酮酸（ＰＥＰＣ）活性变化趋势基本一致。同时,其活性也有昼夜变化,白天活性高,夜间活性低。经水分胁迫诱导出ＣＡＭ 后,ＮＡＤ－ＭＥ活性增加了２—３ 倍。我们认为,ＣＡＭ的调节是由羧化系统的ＰＥＰＣ和脱羧系统的ＮＡＤ－ＭＥ协调作用的结果     

重离子束对酵母细胞的失活与突变

双倍体酵母细胞Ｄ７经单核能为１１．４ＭｅＶ／ｕ的Ａｎ和Ｕ离子辐照后,测定了细胞随剂量的存活率和突变率。获得细胞对Ａｕ和Ｕ离子的失活截面分别为２．５４μｍ２和１．９２μｍ２。在存活率为３７％的条件下,Ａｕ、Ｕ离子的ＲＢＥ分别为０．２８和０．１９。在突变实验中,研究了ＤＮＡ断链后的重组与倒位,它们对Ａｕ和Ｕ离子的截面为：８．３×１０－２μｍ２［σｍ－ｒｅｃ（Ａｕ）］,９．５×１０－５μｍ２［σｍ－ｒｅｃ（Ｕ）］和６．１×１０－４μｍ２［σｍ－ｒｅｖ（Ａｕ）］和３．８×１０－５μｍ２［σｍ－ｒｅｖ（Ｕ）］．最后,对所获结果进行了讨论。     

Karyometric observations of WISH cell cultures irradiated with 3 GHz microwaves.

WISH cell cultures 24 hours after passage were irradiated with 3 GHz microwaves (10 cm) at far field conditions in free space (anechoic chamber) for 30 minutes, at field power density 5 or 20 mW/cm2. Within 1,24 and 48 hours of the exposure to microwave fields the volumes of nuclei and nucleoli were measured with the use of a micrometer, and logvolumes and nucleo-nucleolar ratios were calculated. Under the applied irradiation conditions the culture medium temperature did not exceed 37 degrees C. In cultures irradiated at field power density 20 mW/cm2 increased number of cells with small nuclei and enlarged nucleoli was noted within 1 hour of the exposure. Within 24 and 48 hours after irradiation the nucleolar volume showed a slight decrease, whereas the nuclear volume increased. In cultures irradiated at field power density 5 mW/cm2 increased numbers of cells with enlarged nuclei and nucleoli were found. Analysis of the distribution curves of nuclear and nucleolar volumes suggests that non-thermal power densities of microwaves stimulate the metabolism of cell cultures. However, at higher power densities (20 mW/cm2) the stimulation phase is preceded by a period of reduced viability of cell cultures.     

Microwaves (2,450 MHz) suppress murine natural killer cell activity

The effect of 2,450-MHz CW microwaves on natural killer (NK) cell activity and lymphocyte responsiveness to mitogen stimulation was studied in mice. Groups of mice were irradiated at power densities of 5, 15, or 30 mW/cm2 (SAR = 3.5, 10.5, and 21 W/kg respectively) for 1.5 h on 2 or 9 consecutive days. NK cell activity was determined using an in vitro 51Cr release cytotoxicity assay and an in vivo tumor-cell clearance assay. No consistent change was observed in the mitogen response of spleen cells from sham compared with irradiated mice. A significant suppression of NK cell activity measured in vitro was observed for mice irradiated at 30 mW/cm2, but not at 15 or 5 mW/cm2. A significant suppression of NK cell activity, as determined using the in vivo tumor clearance assay, was also observed at 30 mW/cm2. NK cell activity, as determined using the in vitro assay, returned to normal within 24 h following the last irradiation. Treatment of mice with hydrocortisone caused suppression of NK cell activity measured in vitro and in vivo. Paradoxically, peritoneal macrophage phagocytosis was enhanced following irradiation at 30 mW/cm2, the power density at which NK activity was suppressed. The possible role that microwave heating plays in producing these effects is discussed.     

Microwave exposure alters the expression of 2-5A-dependent RNase

The effects of 2.45-GHz continuous-wave microwaves (SAR = 130 mW/g) on the expression of the interferon-regulated enzymes 2'-5'-oligoadenylate (2-5A) synthetase(s) and 2-5A-dependent endoribonuclease (RNase L) were studied in murine L929 cells. Cells growing as monolayers were removed from the substratum and placed in suspension culture for a 4-h sham or microwave exposure. The cells were returned to monolayer growth for 18 h, and then harvested and assayed to determine the amount of RNase L protein (via [32P]2-5A binding) and the specific activities of RNase L and 2-5A synthetase. Binding of radioactive 2-5A to RNase L for sham- and microwave-exposed samples was 14.5 and 36.4% above control, respectively (the microwave-exposed bound 19.0% more probe than the sham-exposed). The increases in 2-5A binding were accompanied by corresponding elevations of RNase L specific activity. In contrast, sham or microwave irradiation produced no alterations in 2-5A synthetase specific activity. No detectable differences were noted in the postexposure cell viability, plating efficiency, or proliferation rate. Also, there were no detectable differences in cell viability or plating efficiency between controls and cultures irradiated for 2 h when the temperature was simultaneously increased to above normal physiological limits (39 to 45 degrees C). The SAR (130 mW/g) and the power density (95 mW/cm2) used for the greater part of this study were nearly 20 times higher than the ANSI limit of 8 mW/g and 5 mW/cm2 for any 1 g of exposed human tissue.     

半导体激光对紫球藻生物学效应的影响

采用波长650nm,功率40mW,功率密度13W／cm^2的半导体激光,对紫球藻（Porphyridium cruentum)进行诱变,辐照时间分别为5min、10min、20min。通过对紫球藻每天细胞数、叶绿素a、第7d细胞干重和胞外多糖产量的测定可知：与对照组比较,3个处理对紫球藻生长及胞外多糖产生影响,5min、10min均有不同程度的促进作用,其中5min作用最明显,而20min则有抑制作用。     

He-Ne激光对大鼠离体颈上神经节后神经元膜电导的影响

应用细胞内生物电记录技术 ,观测不同功率、不同照射时间的 He- Ne激光 (脉冲频率 1Hz)对大鼠离体颈上神经节后神经元快兴奋性突触后电位 (f- EPSP)期间膜电导的影响。功率密度为 2 m W/ cm2 的 He- Ne激光在照射初期 (1min～ 2 min)引起快兴奋性突触后电位 (f- EPSP)幅值增大 ,同时膜电导增大 ;而在激光照射后期 (后 3m in～8m in)引起节后神经元膜电导减少。功率密度为 5 m W/ cm2 的 He- Ne激光照射期膜电导无明显变化 .结果表明 :功率密度为 2 m W/ cm2 的 He- Ne激光照射初期引起膜电导 (Gl=34.6± 5 .4 n S)较照射前 (Gf=2 6 .8± 6 .2 n S)有明显增大 (P<0 .0 5 ) ,照射后期膜电导减少。提示 :He- Ne激光照射可能是通过两时相效应改变节后神经元膜电导来影响交感神经节内兴奋传递过程。这可能是低功率激光对神经细胞的一种作用机制。     

Leukocyte numbers during the humoral and cell-mediated immune response of Japanese quail after microwave irradiation in ovo

1. Coturnix coturnix japonica eggs were exposed to 2.45-GHz continuous wave microwave radiation at an incident power density of 5 mW/cm2 (SAR = 4 mW/g) during the first 12 days of embryogeny. After hatching, leukocyte differential changes were measured in response to an injection with Alectoris graeca chukar red blood cells (CRBC) and in response to a phytohemagglutinin (PHA) injection in irradiated and nonirradiated (sham) quail of both sexes. 2. Microwave irradiation did not affect anti-CRBC hemagglutinin titers, PHA-evoked dermal swelling or leukocyte numbers and percentages. 3. In both the irradiated and sham irradiated males, lymphocyte percentages decreased while heterophil percentages increased after CRBC or PHA injection. 4. In ovo irradiation with microwaves did not alter the time course of either a humoral immune response or a cell-mediated immune response in Japanese quail.     

In vitro microwave effects on human neutrophil precursor cells (CFU-C)

Human marrow cells were irradiated with 2450-MHz CW microwaves in a fluid-filled waveguide irradiation system. Cell exposure was conducted by placing a marrow cell suspension in 20-μl glass microcapillary tubes that were positioned in the exposure chamber, and irradiated at power densities from 31 to 1,000 mW/cm² (with corresponding specific absorption rates of 62 to 2,000 mW/g) for 15 minutes. The temperature of the sample was maintained at a fixed point. Sham-irradiated (SI) and microwave-irradiated (MWI) cells were cultured in a methylcellulose culture system for neutrophil colony proliferation. There was no reduction in neutrophil colony number on days 6–7 or 12–14 in cells exposed at 31 or 62 mW/cm², but as the power density was increased to 1,000 mW/cm², there was a reduction in colony number of MWI cells compared with SI cells. The microwave interaction with the human neutrophil colony-forming cells was apparently not related to temperature rise, or to the state of cell cycle, and was irreversible.     

Hematologic and immunologic effects of pulsed microwaves in mice

Mice were exposed in the far field in an anechoic chamber to 2,880-MHz pulsed microwaves 3 to 7.5 h daily, 5 days/week for 60 to 360 h. Three experiments were performed at average power densities of 5 mW/cm2 and six at 10 mW/cm2, corresponding to averaged specific absorption rates (SARs) of 2.25 and 4.50 mW/g, respectively. Each experiment consisted of eight mice, with a concurrently sham-exposed group of eight. In two of three studies at 5 mW/cm2, there was a significant increase in bone marrow cellularity in the microwave-exposed groups compared to the sham-exposed groups. Significant differences were occasionally seen in erythrocyte, leukocyte, and platelet values from microwave-exposed groups, but were not consistently observed. In one of six groups exposed at 10 mW/cm2, mean bone marrow cellularity was reduced significantly in the microwave-exposed mice; in another group, the lymphocyte count was increased. In only one exposure (10 mW/cm2 for 360 h) was any significant effect noted on serum proteins: a reduction to 5.1 +/- 0.3 g/dl in the exposed versus 5.6 +/- 0.4 g/dl in the sham-exposed mice. This was due to a decrease in alpha and beta globulins, with no effect on albumin or gamma globulin concentrations. No effect on bone marrow granulocyte/macrophage colony-forming units (CFU) was revealed following exposure of mice to pulsed microwaves at 5 mW/cm2. In one of four exposures at 10 mW/cm2, there was a significant increase in CFU-agar colonies. No significant effects of exposures at 10 mW/cm2 were observed on in vivo and in vitro assays of cell-mediated immune functions. No exposure-related histopathologic lesions were found from examination of several tissues and organs. Results of these series of exposures of mice at SARs of 2.25 and 4.50 mW/g indicated no consistent effects on the hematologic, immunologic, or histopathologic variables examined.     

The in vivo effects of 2.45 GHz microwave radiation on rabbit serum components and sleeping times

Summary An investigation was conducted to determine the effects of relatively low power density microwave exposures on various serum components of the Dutch rabbit. Both continuous wave and pulsed mode exposures at 2.45 GHz were used at power densities of 25, 10 and 5 mW/cm². Studies of 10 serum components were performed. Additional studies were conducted on changes in sleeping times of pentobarbital-sedated rabbits at various power densities. Gross and histopathological examinations were performed on representative samples of animals.Changes in the blood chemistry of irradiated animals were consistent with a dose-dependent response to a non-specific thermal stress at all power densities used. Observed physiological response, as well as rectal temperature measurements, indicated that the thermoregulatory capability of the rabbits was sufficient to compensate for the thermal burden at 5 and 10 mW/cm², but could be overridden by a 2 h exposure at 25 mW/cm². Pathology findings included a mild, repairable nephrosis in animals exposed at a power density of 25 mW/cm².A further investigation of analeptic effects at power densities varying from 5 mW/cm² to 50 mW/cm² resulted in a statistically significant decrease in sleeping times, apparently proportional to power density below 15 mW/cm².This research was partially supported by the US Army Medical Research and Development Command, Contract No. DADA17-72-C-2144. (The views expressed are those of the authors and do not necessarily reflect those of the Department of the Army)     

Tests of mutagenesis and reproduction in male rats exposed to 2,450-MHz (CW) microwaves

Tests of mutagenesis and reproduction were conducted in male rats which were irradiated by 2,450-MHz, continuous-wave (CW) microwaves, 4 hr/day from day 6 of gestation to 90 days of age at 5 mW/cm²; or 5 hr/day for five days beginning on the 90th day of age at 10 mW/cm²; or 4 hr/day, 5 days/ wk for four weeks, beginning on the 90th day of age. During selected weekly periods after treatment, the rats were bred to pairs of untreated, normal female rats that were examined in late pregnancy by means of the dominant lethal assay. The reproductive efficiency of these males, as reflected in their breeding, was also examined for changes relating to their microwave experience. No significant evidence of germ-cell mutagenesis was detected when data of microwave-exposed males were compared with those of sham-exposed males, even though there were significant increases in rectal and intra-testicular temperatures at a power density of 28 mW/cm². Temporary sterility, as indexed by fewer pregnancies, was seen at the highest power density.