鸟氨酸脱羧酶活性微量测定法

本文采用一种简单,微量反应系统,根据 ¹⁴C-鸟氨酸释放的 ¹⁴CO₂量测定鸟氨酸脱羧酶(ODC)的活性,酶反应在置于液闪计数瓶内的玻璃小管中进行,释放的 ¹⁴CO₂被瓶内滤纸片上的海胺吸收。实验结果表明,加酸释放 ¹⁴CO₂后30分钟 ¹⁴CO₂吸收已达最大值,且吸收量与释放量成正比,酶反应测定证明 ¹⁴CO₂释放速度在40分钟内保持恒定。ODC活性与酶浓度呈线性关系,此方法不仅用于ODC活性测定,而且亦可用于其他脱羧酶活性的测定。     

春玉米-晚稻与早稻-晚稻种植模式碳足迹比较

量化作物生产的碳足迹有助于为农业生态系统温室气体减排提供理论依据。利用生命周期法研究了我国南方地区稻田春玉米-晚稻水旱轮作种植模式和早稻-晚稻连作种植模式下粮食生产的碳足迹,并定量分析粮食生产过程中各种碳排放源的相对贡献。结果表明,与早稻-晚稻的连作模式相比,春玉米-晚稻轮作模式的单位面积碳排放降低了6724 kg CO₂-eq/hm²,单位产量的碳足迹降低了0.56 kg CO₂-eq/kg。春玉米比早稻少排放6228 kg CO₂-eq/hm²;与早稻-晚稻模式中晚稻碳排放相比,春玉米-晚稻轮作模式晚稻碳排放降低了497 kg CO₂-eq/hm²。早稻-晚稻种植模式的碳足迹主要来源于甲烷（CH₄）,其碳排放为9776 kg CO₂-eq/hm²（54.8%）,氮肥生产和施用的碳排放为2871 kg CO₂-eq/hm²（16.1%）,灌溉电力消耗的碳排放2849 kg CO₂-eq/hm²（16.0%）。春玉米-晚稻轮作模式的碳足迹主要来源于CH₄的碳排放4442 kg CO₂-eq/hm²（39.9%）,氮肥生产和施用的碳排放2871 kg CO₂-eq/hm²（25.8%）,灌溉电力消耗的碳排放1508 kg CO₂-eq/hm²（13.6%）。该模式中晚稻的碳足迹组成情况与春玉米-晚稻模式的碳足迹相似。但是,对于春玉米而言,其碳足迹主要来源氮肥生产和施用的碳排放1436 CO₂-eq/hm²（50.1%）,氧化亚氮（N₂O）的碳排放为579 kg CO₂-eq/hm²（20.2%）,CH₄的碳排放为378 CO₂-eq/hm²（13.2%）。同时,相比于早稻-晚稻中晚稻的产量（6333 kg/hm²）,春玉米-晚稻轮作模式下的晚稻产量（7270 kg/hm²）提高了14.8%。因此,引入春玉米-晚稻轮作模式有利于提升稻田生产力,降低稻田连作系统碳排放和碳足迹。     

Combined effects of atmospheric CO<Subscript>2</Subscript> and N availability on the belowground carbon and nitrogen dynamics of aspen mesocosms

It is uncertain whether elevated atmospheric CO₂ will increase C storage in terrestrial ecosystems without concomitant increases in plant access to N. Elevated CO₂ may alter microbial activities that regulate soil N availability by changing the amount or composition of organic substrates produced by roots. Our objective was to determine the potential for elevated CO₂ to change N availability in an experimental plant-soil system by affecting the acquisition of root-derived C by soil microbes. We grew Populus tremuloides (trembling aspen) cuttings for 2 years under two levels of atmospheric CO₂ (36.7 and 71.5 Pa) and at two levels of soil N (210 and 970 μg N g^–1). Ambient and twice-ambient CO₂ concentrations were applied using open-top chambers, and soil N availability was manipulated by mixing soils differing in organic N content. From June to October of the second growing season, we measured midday rates of soil respiration. In August, we pulse-labeled plants with ¹⁴CO₂ and measured soil ¹⁴CO₂ respiration and the ¹⁴C contents of plants, soils, and microorganisms after a 6-day chase period. In conjunction with the August radio-labeling and again in October, we used ¹⁵N pool dilution techniques to measure in situ rates of gross N mineralization, N immobilization by microbes, and plant N uptake. At both levels of soil N availability, elevated CO₂ significantly increased whole-plant and root biomass, and marginally increased whole-plant N capital. Significant increases in soil respiration were closely linked to increases in root biomass under elevated CO₂. CO₂ enrichment had no significant effect on the allometric distribution of biomass or ¹⁴C among plant components, total ¹⁴C allocation belowground, or cumulative (6-day) ¹⁴CO₂ soil respiration. Elevated CO₂ significantly increased microbial ¹⁴C contents, indicating greater availability of microbial substrates derived from roots. The near doubling of microbial ¹⁴C contents at elevated CO₂ was a relatively small quantitative change in the belowground C cycle of our experimental system, but represents an ecologically significant effect on the dynamics of microbial growth. Rates of plant N uptake during both 6-day periods in August and October were significantly greater at elevated CO₂, and were closely related to fine-root biomass. Gross N mineralization was not affected by elevated CO₂. Despite significantly greater rates of N immobilization under elevated CO₂, standing pools of microbial N were not affected by elevated CO₂, suggesting that N was cycling through microbes more rapidly. Our results contained elements of both positive and negative feedback hypotheses, and may be most relevant to young, aggrading ecosystems, where soil resources are not yet fully exploited by plant roots. If the turnover of microbial N increases, higher rates of N immobilization may not decrease N availability to plants under elevated CO₂. Received: 12 February 1999 / Accepted: 2 March 2000     

一种测定SOD活力的新方法——碱性二甲基亚砜-鲁米诺化学发光法

本文介绍一种测定SOD(超氧化物歧化酶)活力的新的碱性二甲基亚砜——鲁米诺化学发光法。用碱性二甲基亚砜作为产生O₂^-_·体系,用鲁米诺作为指示O₂^-_·的化学发光剂,观察了不同浓度的NaOH、鲁米诺、pH、碱性二甲基亚砜加入量、测定时间及心绿染料对此法的影响。测定了山羊烟雾吸入伤后SOD活力和肺淋巴SOD清除量的变化。结果证明,本法灵敏度高、特异性强、操作简便、方法稳定,可快速、重复测定粗提取生物样品的SOD活力。     

地质封存CO2泄漏对玉米根系形态的影响

碳捕集与封存（Carbon Capture and Storage,CCS）是应对全球气候变化、实现煤炭清洁利用的有效手段之一,但是地质封存的CO₂存在泄漏的风险,可能对农田生态系统产生重大威胁,影响我国粮食安全。根系生长是地上部和地下部相互作用、相互促进的统一过程,其形态特征对作物生产力有显著影响,但CCS泄漏对植物根系的影响评估尚不多见。本文以玉米为研究对象,采用盆栽底部通入CO₂的方法模拟不同CO₂泄漏情景,研究CK（0 g m^-2 d^-1）和G1000（1000 g m^-2 d^-1）和G2000（2000 g m^-2 d^-1）三种泄漏情景下CO₂对玉米根系形态的影响。结果表明：CO₂泄漏对玉米根系形态有明显的影响,随着泄漏量的增大总根长从40290.81 cm减少至21448.18 cm,减少46.77%,其中细根大幅减少;CO₂泄漏造成玉米明显减产,最大减产率达26.64%;玉米的地上部生物量较地下部生物量对CO₂泄漏更加敏感。综合来看,随着CO₂泄漏量增大,对玉米根的生长、地上部生物量、地下部生物量以及产量有显著的抑制作用。作物根系形态对封存CO₂泄漏的响应可为CCS泄漏监测和生态修复提供系统科学依据。     

若尔盖高原沼泽湿地CO2排放时空变化特征

为了更好理解若尔盖高原不同微生境下沼泽湿地生态系统CO₂排放通量的变化特征,以若尔盖高原湿地自然保护区为研究对象,2013和2014年生长季期间,采用了静态箱和快速温室气体法原位观测了3种湿地5种微生境下沼泽湿地CO₂排放通量时空变化规律。结果表明：长期淹水微地貌草丘区湿地（PHK）和洼地区湿地（PHW） CO₂排放通量变化范围分别为38.99-1731.74 mg m^-2 h^-1和46.69-335.22 mg m^-2 h^-1,季节性淹水区微地貌草丘区湿地（SHK）和洼地区湿地（SHW） CO₂排放通量变化范围分别为193.90-2575.60 mg m^-2 h^-1和49.93-1467.45 mg m^-2 h^-1,而两者过渡区的无淹水区沼泽湿地（Lawn） CO₂排放通量变化范围194.20-898.75 mg m^-2 h^-1。相关性分析表明5种微地貌区沼泽湿地CO₂排放通量季节性变化与不同深度土壤温度均存在显著正相关,与水位存在显著负相关（PHW、SHW、SHK、Lawn）或不相关（PHK）,并且水位和温度（5 cm）共同解释了CO₂排放通量季节性变化的87%。3种湿地5种微生境下沼泽湿地CO₂排放通量存在空间变化规律,主要受水位影响,但植物也影响沼泽湿地CO₂排放通量空间变化规律,并且表明沼泽湿地CO₂排放通量与水位平均值存在显著负相关。     

不同CO2浓度升高和氮肥水平对水稻叶绿素荧光特性的影响

为研究不同CO₂浓度升高和氮肥水平对水稻叶绿素荧光特性的影响,利用由开顶式气室（OTC）组成的CO₂浓度自动调控平台开展田间试验。以粳稻9108为试验材料,CO₂浓度设置CK（对照,环境大气CO₂浓度）、C₁（CO₂浓度比CK增加160 μmol/mol）和C₂（CO₂浓度比CK增加200 μmol/mol）3个水平;氮肥设置低氮（N₁：10 g/m²）、中氮（N₂：20 g/m²）和高氮（N₃：30 g/m²）3个水平。结果表明,在低氮条件下,与CK相比,C₁处理使拔节期的F_o上升4.8%（P=0.031）;C₂处理使拔节期的F_o上升6.3%（P=0.015）,F_v/F_m下降4.8%（P=0.003）,使孕穗期的F_o上升12.7%（P=0.039）,F_v/F_o下降18.2%（P=0.039）。在高氮条件下,与CK相比,C₂处理使灌浆期的F_m、F_v和F_v/F_m分别下降3.6%（P=0.039）、4.9%（P=0.013）和1.3%（P=0.039）。在中氮条件下,与CK相比,C₁和C₂处理的影响不明显。在整个生育期内,CO₂浓度升高与施氮处理交互作用对水稻叶绿素荧光特性的影响未到达显著水平。研究表明,大气CO₂浓度升高使水稻叶片光系统Ⅱ受损,抑制其电子传递能力、电子受体Q_A氧化还原情况、最大光化学效率和潜在活性,通过适量施氮可以有效地缓解其负面效应。     

大鼠前脂细胞质膜Na+/H+交换同时参与细胞的增殖和分化

以原代培养的大鼠前脂细胞为模型 ,以 2′ ,7′ bis ( 2 carboxyethyl) 5 ( 6 ) carboxyfluorescein (BCECF)作为检测胞内pH(pHi)的荧光探针 ,测定不同生长因子刺激下胞内pH的变化 ,证明大鼠肾周前脂细胞质膜存在Na⁺/H⁺交换活性 ,胎牛血清(FCS)能快速激活Na⁺/H⁺交换 ,导致pHi升高 (约 0 .2pH单位 ) ,并引起DNA合成 .Ethyl isopropyl amiloride (EIPA)抑制Na⁺/H⁺交换与DNA合成 .在无血清条件下 ,胰岛素不刺激DNA合成但引起细胞分化 ,表现为胞内脂滴积累和 3 磷酸 甘油脱氢酶(G₃ PDH酶 )活性增强 ,同时激活Na⁺/H⁺交换活性导致pHi升高 ;EIPA既抑制胰岛素对Na⁺/H⁺交换的激活 ,也抑制G₃ PDH酶活性增强 .结果证明 :Na⁺/H⁺交换的激活不仅与大鼠前脂细胞增殖相关 ,同时也是细胞分化的早期事件 .     

室内CO2浓度、温湿度和光照变化对碰碰香挥发物释放量的影响

碰碰香(Plectranthus hadiensis var. tomentosus)的芳香气味具有改善身心健康的作用,但其挥发物的释放易受到室内环境影响而降低效果。为探究碰碰香挥发物对常见室内环境变化的响应,并为其高效稳定地应用于构建舒适的亲生物环境提供科学依据,该研究采用混合正交设计,使用动态顶空和气相色谱质谱联用技术测定了碰碰香挥发物对温度、湿度、CO₂浓度及光照这4种常见室内环境因素的响应。结果表明:(1)在温度、湿度、CO₂浓度和光照4个环境因素中,CO₂浓度和温度对碰碰香植株挥发物释放量的影响较大,而湿度和光照的影响较弱。(2)正常光周期下培养的碰碰香,在夜晚无光照时,CO₂浓度500 μmol·mol^-1、温度25 ℃和湿度60%的环境条件最适于碰碰香植株释放挥发物。此环境条件下碰碰香挥发物的释放总量为86.23 μg·L^-1·kg^-1, 具有改善身心健康的活性成分含量为78.03 μg·L^-1·kg^-1。综上所述,应用碰碰香构建室内亲生物环境,维持或改善人员身心健康时,应主要注意控制CO₂浓度和温度相关的环境条件,从而充分高效地发挥碰碰香的园艺效益。     

Avocado shoot culture, plantlet development and net CO2 assimilation in an ambient and CO2 enhanced environment

Summary The proliferation and survival of avocado nodal cultures of juvenile origin were affected by the form and concentration of nitrogen. Optimum growth was achieved on modified Murashige and Skoog medium containing 67% KNO₃ and 33% NH₄NO₃ with total N of 40 mM supplemented with 100 mg l⁻¹ myo-inositol, 1 mg l⁻¹ thiamine HCl, 30 g l⁻¹ sucrose, and 4.44 μM BA with a 16-h photoperiod (120–150 μmol m⁻² s⁻¹). Proliferating shoots and plantlets were photosynthetically active. Better shoot growth and accumulation of higher biomass occurred in a CO₂-enriched environment than under ambient CO₂ conditions. CO₂ assimilation efficiency, however, was higher under the latter conditions than in a CO₂-enhanced environment, e.g., 31±7 and 17±2 μmol CO₂ m⁻² s⁻¹, respectively. The net CO₂ assimilation rates of in vitro grown plantlets were comparable to those of seedlings ex vitro.     

DISTRIBUTION OF CHOLINE ACETYLTRANSFERASE AND GLUTAMATE DECARBOXYLASE WITHIN THE SUBSTANTIA NIGRA AND IN OTHER BRAIN REGIONS FROM CONTROL AND PARKINSONIAN PATIENTS

—The distribution of choline acetyltransferase (ChAc, EC 2.3.1.6) and l -glutamate 1-carboxylyase (glutamate decarboxylase, GAD, EC 4.1.1.15) was studied in serial frontal slices of the substantia nigra (SN) (pars compacta, PC; pars reticulata, PR; an intermediate region, IR) as well as in other brain areas from post mortem tissue of control and Parkinsonian patients. Within the SN from control brain ChAc and GAD activities showed a distinctive distribution: ChAc activity in PC was higher than in PR and IR by 427% and 253% respectively and within PC the enzyme activity in the rostral part exceeded that in the control part by 353%. The GAD activity in PC was higher by 41% than that in PR and within PC seemed to be higher in the caudal than in the rostral part. For both enzyme activities there were no significant differences between PR and IR or within these regions. In Parkinsonian brain both ChAc and GAD activities were reduced to 15-25% of controls in all 3 regions of the SN. The distinctive distribution of ChAc and GAD activity found in the SN of control brain was abolished: no difference was observed between the 3 regions. However, within PC the ChAc activity was lower in the medial than in the rostral part. Since nigral ChAc is possibly located in interneurons, the decrease in enzyme activity may be connected with the cell loss observed in the SN of Parkinsonian brain. By contrast, nigral GAD is probably contained in terminals of strio-nigral neurons and the decrease in enzyme activity in Parkinson's disease in the absence of striatal cell loss, may reflect a change in the functional state of these GABA neurons. Among various areas of control brains ChAc activity was highest in caudate nucleus and putamen while GAD was highest in SN. caudate nucleus, putamen and cerebral cortex. In Parkinsonian brain the most severe reduction in ChAc and GAD activities was found in the SN.     

THE ROLE OF GABA METABOLISM IN THE CONVULSANT AND ANTICONVULSANT ACTIONS OF AMINOOXYACETIC ACID

Abstract— At high dosage levels AOAA acted as a convulsant agent in mice and rats but in lower amounts it was an effective anticonvulsant agent against INH-induced seizures, by tripling the time to the onset of the convulsions. AOAA elevated brain GABA levels as a result of a preferential inhibition of the GABA-T enzyme system but, contrary to previous reports, the activity of the GAD enzyme system was also inhibited, even by relatively low dosage levels of AOAA. The state of excitability of the brain following the administration of AOAA was related, within the limits of the present study, to changes in GAD activity and GABA levels, but additional data are required before the relationship can be properly evaluated.     

Glutamate decarboxylase activity in chick brain and retina

We have studied the effect of Triton-X-100 on glutamate decarboxylase (GAD) activity in brain and retina from chick embryos of 12 and 16 days' incubation and from chicks 4–6 weeks old. GAD activity was measured in five different homogenization media. Triton-X-100 inhibited the enzyme by about 60% in both brain and retina of 12-day embryos and by about 50% in 16-day embryos, independently of the homogenization medium. In chicks only about 20% inhibition by the detergent was observed in brain whereas no effect was found in retina. These results indicate that the evaluation of the experimental conditions of enzyme assays at different ages is essential for developmental studies of GAD activity in nervous tissue.     

POST MORTEM STABILITY AND STORAGE IN THE COLD OF BRAIN ENZYMES

Tyrosine hydroxylase (TH), glutamate-decarboxylase (GAD) and choline acetyltransferase (CAT) were estimated in the striatum of rat brains kept at 20°C or 4°C for various periods of time up to 48 h after death. At 20°C TH and GAD activities decreased up to 4&50% of controls after 48 h; CAT activity was not affected. Maintenance of dead animals at 4°C completely (GAD and CAT) or partially (TH) prevented the decrease in enzyme activities. In a second series of experiments, TH, G A D and CAT activities were measured in striata (tissue or homogenate) stored immediately after death at different temperatures (4°C; -35°C; -70°C) for various time intervals up to 3 months. Storage of striata at 4°C induced a rapid decrease of all enzyme activities with time (GAD > CAT > TH). TH, GAD and CAT activities in striata kept at -35°C or -70°C were fairly stable. However, CAT activity was slightly decreased when the dissected striata were not homogenized; GAD activity was substantially reduced after 3 months at -35°C. Stability of TH, GAD and CAT activities were confirmed in homogenates of human caudate nucleus stored at -70°C for 1 month. If human enzymes behave similarly to the rat enzymes the following conclusions should be drawn: (1) brains should be obtained at autopsy within 8 h after death; (2) placement of dead bodies in the refrigerator should be done as soon as possible; (3) dissected brain structures (preferably as homogenates) should be stored at -70°C.     

An endogenous activator of renal glutamic acid decarboxylase effects of adenosine triphosphate, phosphate and chloride on the activity of this enzyme.

The renal glutamic acid decarboxylase (GAD) differs from the brain and pancreatic enzyme by its strong binding to membranes that is not influenced by detergents. After centrifugation of freshly prepared homogenate of the rat renal cortex, only 10-15% of GAD activity was found in supernatants and 15-30% in pellets. The majority of the GAD activity was lost. The bound GAD was found in the pellet. A thermolabile activator was present in the supernatant, which was not lost on dialysis. Approximately 55% of the total GAD activity was solubilized in homogenates stored for 24 h at 4 degrees C without detergent, whereas in homogenates stored with Triton X-100, the solubilized GAD increased to 80%. This solubilization was decreased by inhibitors of thioproteases such as leupeptin, antipain and trans-epoxysuccinyl-L-leucylamido-(4-guanidino)butane (E-64). Solubilized GAD was applied to DEAE Toyopearl resin and the GAD activator was eluted with 35 mM Pi. GAD was eluted with 250 mM Pi. The effect of ATP on the activity of renal GAD was also different to its effect on brain GAD. ATP is a strong inhibitor of the brain enzyme at physiological concentrations. ATP (and Pi), together with chlorides (another brain GAD inhibitor), stabilize the renal GAD. However, renal GAD was inhibited by ATP in the presence of leupeptin in freshly prepared homogenates. Similarly, ATP inhibits solubilized GAD from homogenates stored without Triton X-100 for 24 h at 4 degrees C, but Pi retains its stabilizing effect in this preparation. A significant finding of the work presented here is the obligatory requirement of an endogenous activator for renal GAD activity. Whether this activator is an enzyme converting the inactive GAD to active enzyme (as hypothesized for brain GAD), or whether it is a protein affecting the activity of renal GAD by binding (as observed for GAD in some plants) remains to be established.     

Response of the cockroach brain gamma-aminobutyric acid system to isonicotinic acid hydrazide and mercaptopropionic acid

The presence of gamma-aminobutyric acid (GABA) as well as glutamic acid decarboxylase (GAD) and GABA-transaminase (GABA-T) enzymes was demonstrated in the cockroach (Periplaneta americana) brain. Isonicotinic acid hydrazide (INH) in vivo (2.19 mumol/g) inhibited brain GAD activity, the inhibition lasted for about 2 hours and the normal activity levels reappeared at 4 h after INH administration. Brain GABA levels increased initially but then declined and were restored to normal levels at 4 h after INH administration. GABA-T activity was strongly inhibited by INH and a total 100% inhibition was observed at 2-3 h following INH treatment. The GABA-T activity, however, began to recover after 3 h but only 37% of the total enzyme activity was released from inhibition. Mercaptopropionic acid (MPA) in vivo (32 micrograms/g) inhibited brain GAD activity and depleted GABA level also. Results indicate that INH response of the cockroach brain GABA system is similar to that reported for the chick brain but differs from that of the mammalian brain.     

Utilization of Plasma Fatty Acid in Rat Brain: Distribution of [14C]Palmitate Between Oxidative and Synthetic Pathways

Radioactivity within individual brain compartments was determined from 5 min to 44 h after intravenous injection of [14C]palmitate into awake Fischer-344 rats, aged 21 days or 3 months. Total radioactivity peaked broadly between 15 min and 1 h after injection, declined rapidly between 1 and 2 h, and then more slowly. In 3-month-old rats, the lipid and protein brain fractions were maximally labeled within 15 min after [14C]palmitate injection, then retained approximately constant label for up to 2 days. Radioactivity in the aqueous brain fraction comprised mainly radioactive glutamate and glutamine, and peaked at 45 min, when it comprised 48% of total brain radioactivity, then decreased to 27% of the total at 4 h, 15% at 20 h, and 10% at 44 h. Percent distribution of radioactivity within the different brain compartments, 4 h after intravenous injection of [14C]palmitate, was similar in 21-day-old and 3-month-old rats, despite higher net brain uptake in the younger animals. The results indicate that about 50% of plasma [14C]palmitate that enters the brain of adult rats is incorporated rapidly into stable protein and lipid compartments. The remaining [14C]palmitate enters the aqueous fraction after beta-oxidation, and is slowly lost. At 4 h after injection, 73% of brain radioactivity is within the stable brain compartments; this fraction increases to 86% by 20 h.     

DIFFERENTIAL EFFECTS OF AGONAL STATUS ON MEASUREMENTS OF GABA AND GLUTAMATE DECARBOXYLASE IN HUMAN POST-MORTEM BRAIN TISSUE FROM CONTROL AND HUNTINGTON''S CHOREA SUBJECTS

Abstract— GABA and its biosynthetic enzyme glutamic acid decarboxylase (GAD) remained remarkably stable for many hours after death in both human putamen obtained at autopsy and in mouse brain stored under conditions simulating the routine handling of human cadavers. GAD activity was profoundly influenced by agonal status in control but not in choreic subjects. Conversely, GABA concentrations were unaffected by the agonal status but showed a significant age-related decline. GAD activity and GABA concentrations were positively correlated in sudden death control cases but not in control cases suffering a protracted terminal illness or in choreic subjects. In choreic putamen there was an approximate 50% reduction in GABA concentration and GAD activity (correcting for agonal status) consistent with the hypothesis that striatal GABA-containing neurones degenerate in this disease. Since GABA concentrations are unaffected by agonal factors they may provide a reliable marker for the integrity of GABA systems provided that control and pathological groups are matched for age and delay in post-mortem sampling.     

Distribution and tissue specificity of glutamate decarboxylase (EC 4.1.1.15).

Abstract— The activity of L–glutamate decarboxylase (EC 4.1.1.15) (GAD) in various mouse tissues was determined by five different methods, namely, the radiometric CO₂ method, column separation, electro–phoretic separation, the filtration method, and amino acid analysis. Results from the latter four methods agreed well, showing that brain had the highest activity, 4.27 nmol/min/mg protein (100%), followed by heart (7.4%), kidney (6.3%) and liver (1.5%). Measurement of brain GAD using the radiometric CO₂ assay method agreed with the other techniques. However, in heart, kidney, and liver, the GAD activities measured by the CO₂ method were about 3–4 times higher than those obtained by the GABA method, suggesting that the CO₂ method does not give a valid measurement of GAD activity in a crude non–neural tissue preparation. GAD activity also was detected in adrenal gland but not in pituitary, stomach, testis, muscle, uterus, lung, salivary gland, or spleen. GAD from brain, spinal cord, heart, kidney and liver were further compared by double immunodiffusion, enzyme inhibition by antibody, and microcomplement fixation using antibody against GAD purified from mouse brain. GAD from brain and spinal cord appear to be identical as judged from the following results: the immunoprecipitin bands fused together without a spur; the enzyme activity was inhibited by anti–GAD to the same extent; and the microcomplement fixation curves were similar in both the shape of the curve and the extent of fixation. No crossreactivity was observed between GAD from heart, kidney or liver and antibody against brain GAD in all the immunochemical tests described above, suggesting that GAD in non–neural tissues is different from that in brain and spinal cord.     

Excretion, Metabolism and Tissue Distribution of A Spin Trapping Agent, α-Phenyl-N-Tert-Butyl-Nitrone (Pbn) in Rats

The objective of this study is using radiolabelled PBN to determine the tissue distribution, excretion, and metabolism of PBN in rats in order to evaluate the effective time to trap free radical in appropriate tissue(s). Our results demonstrated that PBN is rapidly absorbed when it is injected intraperitoneally in the animal. PBN can be used as an effective spin trapping agent for a variety of tissues since it is evenly distributed among a wide range of tissues measured. Since there is no difference in the tissue concentrations and distribution pattern of PBN at 15, 30 and 60min after injection of PBN. it is appropriate to choose any of these time intervals to terminate the experiment and extract the spin adduct. The excretion of PBN, however, is slow. The majority of the radioactivity (70%) was excreted by the first 3 days. Only 5.7% of radioactivity was collected from 3 to 14 days. The remaining 25% of the radioactivity may be in the form of expired ¹⁴CO₂. Trace amounts of radioactivity were recovered in the feces. PBN has probably only one major form of metabolite excreted in the urine. A small amount of the parent compound, however, was also excreted in the urine. The chemical structure of the metabolite(s) is still unknown.