低置式密闭颅窗模型及兔软脑膜微血管观察

低置式密闭颅窗模型及兔软脑膜微血管观察马虹徐镰陈进贵张日新（江苏职工医科大学,南京２１００２９）在脑循环研究中,密闭颅窗以其能对清醒动物软脑膜微血管的动态变化进行直接、连续观察及慢性长期追踪等优点,已成为探讨影响脑循环生理、病理、药理及其他因素的重要...     

一氧化氮合酶的研究进展

一氧化氮是由Ｌ－精氨酸和氧分子在一氧化氮合酶及其辅因子ＮＡＤＰＨ、ＦＡＤ、ＦＭＮ、ＣａＭ和ＢＨ４催化作用生成的;ＮＯＳ分为原生型和诱生型ＮＯＳ,原生型ＮＯＳ活性依赖于胞浆内Ｃａ＾２＋水平,诱生型ＮＯＳ是Ｃａ＾２＋／ＣａＭ非依赖性酶,其活性开关是胞内ｎＮＯＳ ｍＲＮＡ水平,ＮＯＳ可在多个水平被调节;ＮＯＳ可能在心血管疾病的发病中起重要作用。     

高频喷射通气治疗海水淹溺肺水肿时兔肺钙离子超微结构变化

用海水灌注的方法诱导海水淹溺肺水肿（ＰＥ－ＳＷＤ）, 采用高频喷射通气（ＨＦＪＶ） 治疗, 应用血气酸碱分析仪对兔动脉血气酸碱三项指标进行自动检测, 并采用Ｃａ２＋ 超微结构方法观察肺内Ｃａ２＋ 变化。结果表明肺细胞内Ｃａ２＋ 超负荷与ＰＥ－ＳＷＤ发生有关, ＨＦＪＶ 对改善ＰＥ－ＳＷＤ症状有明显作用, 同时, 细胞内Ｃａ２＋ 超负荷状况明显缓解     

α，β－受体阻断剂对大鼠缺氧性脑血管扩张反应的影响

本实验采用堤式颅窗软脑膜微循环实验方法,利用去甲肾上腺素和α,β－受体阻断剂,研究了交感神经在缺氧性脑血管扩张反应（ＨＣＶ）中的作用。去甲肾上腺素（１０－７ｍｏｌ／Ｌ和１０－６ｍｏｌ／Ｌ）对软脑膜微动脉无明显作用。β－受体阻断剂普萘洛尔（局部用药,下同）对ＨＣＶ无明显影响,而用１０－６ｍｏｌ／Ｌ哌唑嗪阻断软脑膜微动脉α－受体可明显增强ＨＣＶ（由２１．５±９．８％增至３０．６±９．２％,Ｐ＜０．０１）。结果提示,正常情况下交感神经对脑血管影响较小,但在缺氧时,交感神经对脑血管有收缩作用。交感神经可能通过增加其末梢释放去甲肾上腺素,作用于α－受体,限制微劝脉扩张而在缺氧性脑血管扩张反应中起调节作用。     

水霉（Saprolegnia ferax）生长菌丝顶端细胞内游离Ca^2＋和膜结合…

本文比较和研究了水霉（Ｓａｐｒｏｌｅｇｎｉａ ｆｅｒａｘ）生长菌丝顶端胞内Ｆｌｕｏ－３游离Ｃａ＾２＋和ＣＴＣ－膜结合Ｃａ＾２＋的荧光分布影像。激光共焦扫描显微镜下观察可见：Ｆｌｕｏ－３荧光有房室化现象,Ｆｌｕｏ－３荧光反映的是细胞质游离Ｃａ＾２＋与细胞器游离Ｃａ＾２＋总的分布状况,Ｆｌｕｏ－３游离Ｃａ＾２＋的最大荧光强度出现在菌丝顶端２－１０ｕｍ区域,１０ｕｍ以后荧光强度逐渐下降,约４０ｕｍ以后荧     

大鼠酰胺化酶的信号肽引导的昆虫细胞表达外泌系统

将大鼠酰胺化酶的信号肽及前导肽编码序列引入昆虫核多角体病毒转移表达载体,构建ＰＡＢＣｈＧＲＦ（Ｇｌｙ）、ＰＡＢＣＩＧＦＩ融合基因的昆虫细胞分泌表达质粒ｐＢａｃＰＡＧ２、ｐＢａｃＰＡＩ,并与经修饰的银纹夜蛾核多角体病毒ＢａｃＰＡＫ６线性化ＤＮＡ共转染秋粘虫细胞Ｓｆ２１,通过同源重组、筛选和鉴定,得到它们的重组病毒ＢａｃＰＡＧ、ＢａｃＰＡＩ。将重组病毒感染Ｓｆ２１细胞,ＰＡＢＣｈＧＲＦ（Ｇｌｙ）和ＰＡＢＣＩＧＦＩ均得到有效外泌表达,表达产物通过ＩｇＧＳｅｐｈａｒｏｓｅ柱可获得快速纯化。     

TFP刺激裂殖酵母细胞钙离子内流的质膜效应

ＴＦＰ（１０－１００μｍｏｌ／Ｌ）可引起裂殖酵母（Ｓｃｈｉｚｏｓａｃｃｈａｒｏｍｙｃｅｓ　ｐｏｍｂｅ）胞外Ｃａ２＋内流,ＴＦＰ浓度不同,促进Ｃａ２＋内流程度也不一样,５０μｍｏｌ／ＬＴＦＰ的促进作用最大。并且ＴＦＰ浓度越大,Ｃａ２＋内流出现峰值也越早,１０、２０、５０、１００μｍｏｌ／ＬＴＦＰ处理后,胞内总钙出现峰值时间分别为４５、４５、３０、１５分钟。胞外Ｈ＋浓度也会对ＴＦＰ引起的Ｃａ２＋内流产生不同影响,缓冲液的ｐＨ值为６．０时最有利于ＴＦＰ引起胞内Ｃａ２＋含量增加,碱性条件下ＴＦＰ的效果最不明显。由ＴＦＰ引起的Ｃａ２＋内流增加要比单一地增加外钙浓度效果好得多,ＴＦＰ在１０μｍｏｌ／Ｌ浓度的外钙条件下引起的胞内钙含量数值比１０００μｍｏｌ／Ｌ的外钙条件而无ＴＦＰＴ所引起的胞内钙含量还要高５３．９％。缓冲液中加入０．８％的钙离子通道阻断剂ＬａＣ１３或溶液中无葡萄糖的存在,ＴＦＰ的促进作用消失,说明ＴＦＰ促进Ｃａ２＋内流是通过钙离子通道来完成的并需要能量参与。     

TFP刺激裂殖酵母细胞钙离子内流的质膜效应*

ＴＦＰ（１０－１００μｍｏｌ／Ｌ）可引起裂殖酵母（Ｓｃｈｉｚｏｓａｃｃｈａｒｏｍｙｃｅｓ　ｐｏｍｂｅ）胞外Ｃａ２＋内流,ＴＦＰ浓度不同,促进Ｃａ２＋内流程度也不一样,５０μｍｏｌ／ＬＴＦＰ的促进作用最大。并且ＴＦＰ浓度越大,Ｃａ２＋内流出现峰值也越早,１０、２０、５０、１００μｍｏｌ／ＬＴＦＰ处理后,胞内总钙出现峰值时间分别为４５、４５、３０、１５分钟。胞外Ｈ＋浓度也会对ＴＦＰ引起的Ｃａ２＋内流产生不同影响,缓冲液的ｐＨ值为６．０时最有利于ＴＦＰ引起胞内Ｃａ２＋含量增加,碱性条件下ＴＦＰ的效果最不明显。由ＴＦＰ引起的Ｃａ２＋内流增加要比单一地增加外钙浓度效果好得多,ＴＦＰ在１０μｍｏｌ／Ｌ浓度的外钙条件下引起的胞内钙含量数值比１０００μｍｏｌ／Ｌ的外钙条件而无ＴＦＰＴ所引起的胞内钙含量还要高５３．９％。缓冲液中加入０．８％的钙离子通道阻断剂ＬａＣ１３或溶液中无葡萄糖的存在,ＴＦＰ的促进作用消失,说明ＴＦＰ促进Ｃａ２＋内流是通过钙离子通道来完成的并需要能量参与。     

大鼠TCF—a修饰16肽的溶液构象

已知大鼠ＴＧＦ－ａ的抗原部位于Ｃ环,且大鼠的ＴＧＦ－ａ（３４－４３）和ＴＧＦａ（４４－５０）均有较强的活性以转化正常细胞。为了提示其结构与功能关系,合成了大鼠ＴＧＦ－ａ修饰１６肽。在前文用二维核磁共振技术归属质子谱并验证其一级结构的基础上,本文测定了不同混合时间的二维ＮＯＥＳＹ谱。根据所得的数据原始斜率法求出距离约束。通过约束分子动力学计算定出该分子溶液构象。其中还用ＤＱＦ－ＣＯＳＹ的数据求出二面     

利用流式细胞术检测线粒体PTP开放

用线粒体电位特异必 光探针Ｒｈｏｄａｍｉｎｅ１２３标记线粒休后,在改装ＦＡＣＳ４２０流式细胞仪上用Ｃ－３０数据集集和储存程序采集并存储数据,用Ｃ－３０分析程序分析得取反映线料体前散射（ＦＳＣ）、Ｒｈｏｄａｍｉｎｅ１２３荧光强度和侧散射（ＳＳＣ） ＦＳＣ,ＦＬ１和ＦＬ２合并图。结果显示,２００μｍｏｌ／ＬＣａ＾２＋处理２０分钟使线粒体同时发生ＦＳＣ增大、Ｒｈｏｄａｍｉｎｅ１２３荧光强度降低和ＳＳＣ增     

Application of Thinned-Skull Cranial Window to Mouse Cerebral Blood Flow Imaging Using Optical Microangiography

In vivo imaging of mouse brain vasculature typically requires applying skull window opening techniques: open-skull cranial window or thinned-skull cranial window. We report non-invasive 3D in vivo cerebral blood flow imaging of C57/BL mouse by the use of ultra-high sensitive optical microangiography (UHS-OMAG) and Doppler optical microangiography (DOMAG) techniques to evaluate two cranial window types based on their procedures and ability to visualize surface pial vessel dynamics. Application of the thinned-skull technique is found to be effective in achieving high quality images for pial vessels for short-term imaging, and has advantages over the open-skull technique in available imaging area, surgical efficiency, and cerebral environment preservation. In summary, thinned-skull cranial window serves as a promising tool in studying hemodynamics in pial microvasculature using OMAG or other OCT blood flow imaging modalities.     

Effects of Bilobalide on Hypoxia/Hypoglycemia-Stimulated Glutamate Efflux from Rat Cortical Brain Slices

The aim of this study was to investigate the effects of bilobalide, the postulated active constituent of Ginkgo biloba, on the release of glutamate elicited by hypoxia/hypoglycemia. Cortical slices were prepared from rat brain and perfused with normal artificial cerebrospinal fluid (aCSF) or aCSF made hypoxic by gassing with nitrogen, and hypoglycemic by removal of glucose. The perfusate was assayed for glutamate by HPLC. After 30 minutes, perfusion with hypoxic/hypoglycemic aCSF glutamate levels in the perfusate were increased approximately 5-fold. Bilobalide at 1, 10, and 100 M, when perfused together with hypoxic/hypoglycemic aCSF, significantly reduced the release of glutamate. This study suggests that the reported neuroprotective properties of bilobalide may, in part, be mediated through its ability to reduce glutamate efflux, thus leading to a decrease in the excitotoxic effects of this neurotransmitter.     

Regulation of flagellar dynein by calcium and a role for an axonemal calmodulin and calmodulin-dependent kinase

Ciliary and flagellar motility is regulated by changes in intraflagellar calcium. However, the molecular mechanism by which calcium controls motility is unknown. We tested the hypothesis that calcium regulates motility by controlling dynein-driven microtubule sliding and that the central pair and radial spokes are involved in this regulation. We isolated axonemes from Chlamydomonas mutants and measured microtubule sliding velocity in buffers containing 1 mM ATP and various concentrations of calcium. In buffers with pCa > 8, microtubule sliding velocity in axonemes lacking the central apparatus (pf18 and pf15) was reduced compared with that of wild-type axonemes. In contrast, at pCa4, dynein activity in pf18 and pf15 axonemes was restored to wild-type level. The calcium-induced increase in dynein activity in pf18 axonemes was inhibited by antagonists of calmodulin and calmodulin-dependent kinase II. Axonemes lacking the C1 central tubule (pf16) or lacking radial spoke components (pf14 and pf17) do not exhibit calcium-induced increase in dynein activity in pCa4 buffer. We conclude that calcium regulation of flagellar motility involves regulation of dynein-driven microtubule sliding, that calmodulin and calmodulin-dependent kinase II may mediate the calcium signal, and that the central apparatus and radial spokes are key components of the calcium signaling pathway.     

Temperature and pH/CO(2) modulate respiratory activity in the isolated brainstem of the bullfrog (Rana catesbeiana)

The effects of temperature and pH/CO(2) were examined in isolated brainstem preparations from adult North American bullfrogs (Rana catesbeiana). These experiments were undertaken to determine the effects of temperature on fictive breathing, central pH/CO(2) chemoreception, and to examine potential alphastat regulation of respiration in vitro. Adult bullfrog brainstem preparations were isolated, superfused with an artificial cerebrospinal fluid (aCSF) and respiratory-related neural activity was recorded from cranial nerves V, X and XII. In Series I experiments (N=8), brainstem preparations were superfused with aCSF equilibrated with 2% CO(2) at temperatures ranging from 10 to 30 degrees C. Neural activity was present in all preparations in the temperature range of 15-25 degrees C, but was absent in most preparations when aCSF was at 10 or 30 degrees C. The absence of fictive breathing at high (30 degrees C) temperatures was transient since fictive breathing could be restored upon returning the preparation to 20 degrees C. In Series II experiments (N=10), preparations were superfused with aCSF equilibrated with 0%, 2% and 5% CO(2) at temperatures of 15, 20 and 25 degrees C. Fictive breathing frequency (f(R)) was significantly dependent upon aCSF pH at all three temperatures, with slopes ranging from -0.82 min(-1) pH unit(-1) (15 degrees C) to -3.3 min(-1) pH unit(-1) (20 degrees C). There was a significant difference in these slopes (P<0.02), indicating that central chemoreceptor sensitivity increased over this temperature range. Fictive breathing frequency was significantly dependent upon the calculated alpha-imidazole (alpha(Im)) ionization (P<0.05), consistent with the alphastat hypothesis for the effects of temperature on the regulation of ventilation. However, most of the variation in f(R) was not explained by alpha(Im) (R(2)=0.05), suggesting that other factors account for the regulation of fictive breathing in this preparation. The results indicate that the in vitro brainstem preparation of adult bullfrogs has a limited temperature range (15-25 degrees C) over which fictive breathing is consistently active. Although there is a close correspondence of ventilation in vitro and in vivo at low temperatures, these data suggest that, as temperature increases, changes in ventilation in the intact animal are likely to be more dependent upon peripheral feedback which assumes a greater integrative role with respect to chemoreceptor drive, respiratory frequency and tidal volume.     

Acute Brain Trauma in Mice Followed By Longitudinal Two-photon Imaging

Although acute brain trauma often results from head damage in different accidents and affects a substantial fraction of the population, there is no effective treatment for it yet. Limitations of currently used animal models impede understanding of the pathology mechanism. Multiphoton microscopy allows studying cells and tissues within intact animal brains longitudinally under physiological and pathological conditions. Here, we describe two models of acute brain injury studied by means of two-photon imaging of brain cell behavior under posttraumatic conditions. A selected brain region is injured with a sharp needle to produce a trauma of a controlled width and depth in the brain parenchyma. Our method uses stereotaxic prick with a syringe needle, which can be combined with simultaneous drug application. We propose that this method can be used as an advanced tool to study cellular mechanisms of pathophysiological consequences of acute trauma in mammalian brain in vivo. In this video, we combine acute brain injury with two preparations: cranial window and skull thinning. We also discuss advantages and limitations of both preparations for multisession imaging of brain regeneration after trauma.     

Utilizing a Cranial Window to Visualize the Middle Cerebral Artery During Endothelin-1 Induced Middle Cerebral Artery Occlusion

Creation of a cranial window is a method that allows direct visualization of structures on the cortical surface of the brain^1-3. This technique can be performed in many locations overlying the rat cerebrum, but is most easily carried out by creating a craniectomy over the readily accessible frontal or parietal bones. Most frequently, we have used this technique in combination with the endothelin-1 middle cerebral artery occlusion model of ischemic stroke to quantify the changes in middle cerebral artery vessel diameter that occur with injection of endothelin-1 into the brain parenchyma adjacent to the proximal MCA^{4, 5}. In order to visualize the proximal portion of the MCA during endothelin -1 induced MCAO, we use a technique to create a cranial window through the temporal bone on the lateral aspect of the rat skull (Figure 1). Cerebral arteries can be visualized either with the dura intact or with the dura incised and retracted. Most commonly, we leave the dura intact during visualization since endothelin-1 induced MCAO involves delivery of the vasoconstricting peptide into the brain parenchyma. This bypasses the need to incise the dura directly over the visualized vessels for drug delivery. This protocol will describe how to create a cranial window to visualize cerebral arteries in a step-wise fashion, as well as how to avoid many of the potential pitfalls pertaining to this method.     

A comparison of hole punch and needle punch methods for the measurement of seagrass productivity

Seagrass productivity, as leaf extension, was measured using the hole punch and needle punch techniques. These methods have been widely implemented to determine seagrass leaf extension rates, yet there is no evidence in the literature of a comparison between methods. The hole punch method involves removing part of the basal area of a seagrass leaf and it was proposed that this measurement technique may affect the leaf extension rates that are being measured. Leaf extension rates were measured in Posidonia sinuosa meadows off the coast of Perth, Western Australia. There were no significant differences in seagrass leaf extension between the two methods. The hole punch method is favoured, as measurement of incremental leaf growth is facilitated by the obvious hole left by the punch. The needle punch method leaves lesions on seagrass leaves that are easily confused with other lesions, possibly left by invertebrate grazers. These findings are likely to be applicable to other straplike seagrass species, though a similar comparison is recommended in the initial stages of a study.     

The inner dynein arms I2 interact with a "dynein regulatory complex" in Chlamydomonas flagella.

We provide indirect evidence that six axonemal proteins here referred to as "dynein regulatory complex" (drc) are located in close proximity with the inner dynein arms I2 and I3. Subsets of drc subunits are missing from five second-site suppressors, pf2, pf3, suppf3, suppf4, and suppf5, that restore flagellar motility but not radial spoke structure of radial spoke mutants. The absence of drc components is correlated with a deficiency of all four heavy chains of inner arms I2 and I3 from axonemes of suppressors pf2, pf3, suppf3, and suppf5. Similarly, inner arm subunits actin, p28, and caltractin/centrin, or subsets of them, are deficient in pf2, pf3, and suppf5. Recombinant strains carrying one of the mutations pf2, pf3, or suppf5 and the inner arm mutation ida4 are more defective for I2 inner arm heavy chains than the parent strains. This evidence indicates that at least one subunit of the drc affects the assembly of and interacts with the inner arms I2.     

Morphological development of the gonads in zebrafish

Gonadogenesis of zebrafish Danio rerio was investigated by means of light microscopy to test the suitability of gonad histology as an endpoint in hazard assessment of endocrine‐active compounds. At age 2 weeks post‐fertilization (pf), primordial germ cells were found in a dorsocaudal position in the body cavity. At 4 weeks pf, the majority of the fish (86%) possessed paired gonads with meiotic germ cells; these gonads represented presumptive ovaries. At week 5 pf, 87% of the fish examined had ovaries with perinucleolar oocytes. Further development of the gonads in female zebrafish up to week 11 pf was characterized by an increase in gonad size as well as in the number and size of perinucleolar oocytes. Starting with week 5, some fish showed alterations of gonad morphology, including a decrease in the number and size of the oocytes, an enhanced basophilia and irregular shape of the oocytes, and finally their degeneration into residual bodies. With the decline in oocyte number, stromal cells became more numerous and they infiltrated the gonadal matrix. In several 7 week‐old zebrafish with altered gonadal morphology, enhanced numbers of gonial cells arranged in cyst‐like groups appeared. These gonads were interpreted as presumptive testes. In one fish out of 32 individuals examined, spermatocytes were detected, in addition to the gonial cells. During the subsequent weeks, the percentage of fish showing early testes with spermatogonia, spermatocytes and spermatids increased and reached 40% at 11 weeks pf. The sequence of gonadal alterations taking place in some of the individuals from week 5 pf onwards was interpreted to reflect the transition of protogynic ovaries into testes. The developmental pattern described identifies zebrafish to be a juvenile hermaphrodite. The results of this study are of relevance for the use of gonadal histopathology as endpoint in endocrine disruption testing, particularly in order to avoid false diagnoses of ‘intersex gonads’ in zebrafish.     

Effects of purified human interleukin-1 on sleep and febrile response of cats

From cats prepared for chronic polygraphic recordings sleep patterns were obtained for 8 hours after: 1) intracerebroventricular (icv) injection of artificial cerebrospinal fluid (aCSF), day 1; 2) icv injection of interleukin-1 (I1-1), day 2; 3) injection of aCSF, 24 h after injection of I1-1, day 3; 4) injection of aCSF, 48 after injection of I1-1, day 4. Three doses of I1-1 were tested. The dose of 10 nmol slightly prolonged sleep, whereas a dose of 40 nmol totally inhibited sleep. Twenty nmol of I1-1 elicited sleep and increased body temperature. Total sleep (TS) time was significantly increased due to the significant increase in non REM (NREM) sleep as compared to the control day 1. REM sleep was also increased, but this increase did not reach statistical significance. Wakefulness (W) was significantly reduced. At this time the cats were febrile. On day 3, a further significant increase in TS occurred. NREM was significantly increased when compared with day 1, whereas the increase in REM sleep was significant when compared to both day 1 and day 2. At this time body temperature was normal. The increase in REM sleep on days 2 and 3 resulted entirely from the significant increase in the number of REM periods. On day 4, W showed tendency to increase while sleeping time decreased; such tendency suggests that sleep increase caused by I1-1 slowly returns to the control levels. Our results, together with the earlier evidence on somnogenic and pyrogenic action of I1-1, suggest that these actions may be temporarily dissociated.