外源脯氨酸对盐胁迫下甜瓜幼苗硝酸还原的影响

采用营养液水培方法,以＂雪美＂品种甜瓜（Cucumis melo L.）为材料,研究了外源脯氨酸（Proline）对盐胁迫下甜瓜幼苗叶片和根系硝酸还原的影响。结果表明：（1）盐胁迫提高了甜瓜幼苗叶片和根系内铵态氮（NH4＋-N）和可溶性蛋白含量;降低了硝态氮（NO-3-N）含量和硝酸还原酶（nitrate reductase,NR）活性。（2）外源施用脯氨酸明显地提高了盐胁迫下甜瓜幼苗叶片和根系内NO-3-N和可溶性蛋白含量;降低了盐胁迫下甜瓜幼苗叶片和根系内NH＋4-N含量;增强了盐胁迫下甜瓜幼苗体内NR活性。研究结果表明,外源脯氨酸可以通过调节甜瓜幼苗体内硝酸还原酶活性和氮化合物含量来缓解盐胁迫对甜瓜幼苗植株的伤害。     

外源亚精胺对不同盐浓度下黄瓜幼苗可溶性蛋白表达的影响

采用营养液水培的方法,以黄瓜品种‘津春2号’为试材,研究了叶片喷施外源亚精胺(Spd)对不同浓度NaCl(0、50、75、100 mmo.lL-1)胁迫下幼苗植株可溶性蛋白表达的影响。结果表明,50 mmol.L-1NaCl胁迫下植株叶片和根系中可溶性蛋白含量提高;75 mmol.L-1和100 mmol.L-1NaCl胁迫明显降低了幼苗植株叶片和根系中可溶性蛋白的含量。不同浓度NaCl胁迫下喷施Spd后可溶性蛋白含量在根系中没有明显变化规律,而叶片可溶性蛋白含量提高。SDS-聚丙烯酰胺凝胶电泳(SDS-PAGE)对黄瓜幼苗根系可溶性蛋白分析表明,至少有3种分子量约为61.5、50、47 kD蛋白在50 mmo.lL-1和75 mmol.L-1NaCl胁迫下表达量增强,但100 mmo.lL-1NaCl胁迫下变化不明显;50 mmol.L-1和75 mmol.L-1NaCl胁迫下喷施Spd后61.5 kD和47 kD蛋白表达量明显减弱,50 kD蛋白甚至消失,100 mmol.L-1NaCl胁迫下61.5 kD和47 kD蛋白无明显变化,50 kD蛋白反而增强。     

氮素形态对黄檗幼苗生长及氮代谢相关酶类的影响

通过改变水培溶液中NH4+-N和NO3--N的比例, 研究了不同氮素形态对黄檗(Phellodendron amurense)幼苗生长及氮代谢相关酶类的影响。结果表明, 硝态氮比例较高的营养供给比铵态氮比例较高的营养供给有利于黄檗幼苗的生长, 叶片叶绿素含量和可溶性蛋白含量也高。在NH4+-N/NO3--N为25/75 时黄檗幼苗具有最大生物量。在铵态氮比例大的营养供给下, 黄檗幼苗的谷氨酰胺合成酶(GS)活性增强,而在硝态氮比例大的营养供给下幼苗的硝酸还原酶(NR)活性则较高, 叶片中的硝态氮较低。营养液的氮素形态及其组成通过影响GS与NR的活性而调控黄檗幼苗的氮素代谢。     

等渗Ca(NO3)2和NaCl胁迫对黄瓜幼苗生长及渗透调节物质含量的影响

采用营养液培养方法,以耐盐性较弱的‘津春2号’黄瓜品种为试材,研究了等渗Ca(NO3)2和NaCl胁迫对黄瓜幼苗生长、根系电解质渗透率、根系活力、Na+和K+含量及渗透调节物质含量的影响。结果显示:(1)在84mmol.L-1 NaCl和56mmol.L-1 Ca(NO3)2等渗胁迫下,黄瓜幼苗鲜重和干重均显著下降,且NaCl处理下降的幅度大于等渗Ca(NO3)2处理。(2)NaCl主要通过对黄瓜根系的伤害来抑制植株生长,表现为根系活力下降、根系质膜透性增大、Na+大量积累、K+含量显著下降、Na+/K+明显上升,最终导致根冠比下降;而Ca(NO3)2处理对根系质膜透性、K+含量、Na+/K+的影响均小于NaCl胁迫,且根系活力和根冠比上升,但Ca(NO3)2胁迫后叶片含水量和渗透调节能力均小于NaCl胁迫。(3)NaCl胁迫条件下,黄瓜幼苗内渗透调节物质以可溶性糖为主,而Ca(NO3)2胁迫以可溶性蛋白为主。研究表明,NaCl胁迫对黄瓜幼苗的伤害大于等渗Ca(NO3)2,NaCl主要通过破坏根系质膜结构影响植株生长,而Ca(NO3)2主要通过引起地上部生理干旱来影响植株生长。     

叶施NO对NaCl胁迫下红砂幼苗叶片和根系中氮代谢酶及营养物质的影响

以当年生红砂(Reaumuria soongorica)幼苗为材料,采用盆栽实验,考察叶面喷施不同浓度(0、0.01、0.10、0.25、0.50、1.00 mmol·L^-1)NO供体硝普钠 (SNP) 对NaCl(300 mmol·L^-1)胁迫下红砂根、叶中可溶性蛋白、游离氨基酸和硝态氮含量,以及谷氨酰胺合成酶(GS)、谷氨酸合酶(GOGAT)、硝酸还原酶(NR)活性的影响,并采用主成分分析和隶属函数法筛选NO对NaCl胁迫缓解效应的氮代谢指标和最佳NO浓度,以探讨外源NO对NaCl 胁迫下红砂缓解效应的氮代谢响应机制。结果表明：(1)在300 mmol·L^-1 NaCl胁迫处理下,红砂幼苗根、叶中可溶性蛋白、硝态氮含量以及GS、GOGAT、NR活性均比对照显著下降。(2)外源NO能显著提高盐胁迫下红砂叶、根中GS、GOGAT、NR活性和硝态氮含量,增加根中可溶性蛋白和游离氨基酸含量。(3)NR和GOGAT活性可用于评价NO对NaCl胁迫下红砂幼苗的缓解作用,外源NO(SNP)对红砂幼苗在NaCl胁迫下的缓解效果强弱表现为0.25 mmol·L^-1> 0.50 mmol·L^-1> 0.10 mmol·L^-1> 1.00 mmol·L^-1> 0.01 mmol·L^-1。研究发现,300 mmol·L^-1 NaCl胁迫显著抑制了红砂幼苗氮代谢,外源NO(SNP)有助于提高盐胁迫下红砂NR活性,加快硝态氮转化为铵态氮,促进红砂叶片和根中GS/GOGAT对转化物的同化,从而增强红砂幼苗的耐盐性,并以0.25 mmol·L^-1SNP处理时缓解作用最佳;NR和GOGAT活性可作为NO缓解盐胁迫的评价指标。     

氯化胆碱对盐胁迫黄瓜幼苗渗透调节物质及活性氧代谢系统的影响

以盐敏感型黄瓜品种津春4号为材料,采用水培方法研究了叶面喷施不同浓度(0.5、1.0和1.5 mmol·L-1)氯化胆碱(CC)对NaCl胁迫(75 mmol·L-1)下黄瓜幼苗鲜重、叶片叶绿素、渗透调节物质含量及活性氧代谢系统的影响.结果表明:(1)单独CC处理可提高黄瓜叶片的叶绿素、可溶性糖和可溶性蛋白含量以及过氧化氢酶(CAT)与过氧化物酶(POD)活性,降低O2·-产生速率,但对植株鲜重及超氧化物岐化酶(SOD)活性影响不大;(2)NaCl胁迫处理增加了黄瓜幼苗叶片中可溶性糖和可溶性蛋白含量,增强了SOD、POD和CAT活性,提高了O2·-产生速率及丙二醛(MDA)的含量,但同时降低了叶绿素含量与植株鲜重;(3)盐胁迫前CC预处理可缓解黄瓜幼苗叶绿素含量和植株鲜重的下降、以及MDA含量和O2·-产生速率的上升趋势,且进一步提高了盐胁迫下黄瓜叶片中SOD、POD和CAT活性.因此,适宜浓度的氯化胆碱可显著提高盐胁迫下黄瓜叶片的抗氧化酶活性,提高清除活性氧的能力,缓解盐胁迫对黄瓜幼苗细胞膜的伤害,增强黄瓜幼苗的耐盐性.     

外源NO对NaCl胁迫下黄瓜幼苗生长和根系谷胱甘肽抗氧化酶系统的影响

以津春2号黄瓜为材料,采用营养液水培的方法,研究了外源一氧化氮(NO)对黄瓜幼苗生长和根系谷胱甘肽抗氧化酶系统的影响.结果表明,(1)正常生长条件下添加NO能促进黄瓜幼苗生长,而添加亚甲基蓝(MB-1)显著抑制黄瓜幼苗的生长;(2)添加NO显著缓解了NaCl胁迫对黄瓜幼苗生长的抑制,提高根系还原型谷胱甘肽(GSH)含量、抗坏血酸过氧化物酶(APX)和谷胱甘肽还原酶(GR)活性,而氧化型谷胱甘肽(GSSG)含量略有下降,同时缓解了NaCl胁迫下抗坏血酸(ASA)含量的下降幅度;(3)NaCl胁迫下添加NO的同时添加MB-1可部分解除NO的作用,与NaCl胁迫下单独添加NO处理比较,GR活性、GSH和ASA含量均降低,GSSG含量提高,APX先升高后下降.研究发现,外源NO可能通过鸟苷酸环化酶(cGC)介导来调节NaCl胁迫下黄瓜幼苗根系GR活性和GSH、GSSG、ASA含量,提高抗氧化酶活性和非酶抗氧化物质含量,增强植株对活性氧的清除能力,减少膜脂过氧化,缓解NaCl胁迫对黄瓜幼苗造成的伤害.     

外源亚精胺对高温胁迫下黄瓜幼苗氮素代谢的影响

以较为耐热的黄瓜品种‘津春4号’为试材,在人工气候箱中,采用石英砂培加营养液浇灌的栽培方式,研究了外源亚精胺( Spd)对高温胁迫(42℃)下黄瓜幼苗氮素代谢的影响.结果表明:短期高温胁迫处理,尤其是4h内,植株硝态氮含量降低而铵态氮含量升高;外源Spd预处理使幼苗体内硝态氮和铵态氮含量升高且硝酸还原酶(NR)活性增强.较长期高温胁迫处理下,幼苗根系中硝态氮含量升高但向地上部运输受阻,根系NR钝化,根系和叶片中铵态氮含量均显著升高;高温胁迫下喷施Spd,除进一步促进根系吸收硝态氮且向地上部运输外,根系和叶片NR活性亦有所升高,从较长期的效果看,外源Spd还具有防止铵态氮过度积累、促进幼苗体内氮素代谢趋于正常的作用.     

生菜硝酸还原酶基因的克隆及高氮水平下外源γ-氨基丁酸对其表达和叶片硝酸盐含量的影响

硝酸还原酶(NR)是硝酸盐代谢的关键酶。该研究在成功克隆生菜NR基因的同时,进行了高氮水平下外源γ-氨基丁酸(GABA)对生菜叶片NR基因表达和NO3--N含量的研究。结果表明:(1)生菜NR基因(GenBank登录号为KP122207)序列长1 791bp,编码585个氨基酸残基,蛋白保守结构域含钼辅蛋白超家族、细胞色素b5超家族和FNR超家族;生菜NR基因与菊苣NR基因亲缘关系最近,序列一致性为93%,与烟草、甜菜、黄瓜、大豆等NR序列的一致性均在80%以上。(2)高氮水平下外源2.5mmol/L GABA处理生菜可诱导NR基因上调表达,并显著提高了生菜叶片NR、亚硝酸还原酶(NiR)、谷氨酸脱羧酶(GAD)活性和NH4+-N含量,降低了NO3--N、NO2--N含量;虽然NO3--N含量与NR、GAD、NiR活性、NO2--N、NH4+-N含量均呈显著相关关系,但与NR活性的相关系数最高且达极显著水平。研究认为,高氮水平下外源GABA可通过诱导NR基因上调表达、增强相关酶活性来影响无机氮代谢,从而降低了生菜叶片硝酸盐含量,其中NR在该过程中发挥着至关重要的作用,为生产中GABA的施用及降低叶菜类蔬菜硝酸盐含量提供了理论依据。     

外源GSH对盐胁迫下番茄幼苗生长及抗逆生理指标的影响

采用营养液栽培法,研究外源谷胱甘肽(GSH)对NaCl胁迫下番茄幼苗生长、根系活力、电解质渗透率和丙二醛(MDA)、脯氨酸(Pro)、可溶性糖含量以及超氧化物歧化酶(SOD)、过氧化物酶(POD)、过氧化氢酶(CAT)活性的影响,为利用外源物质减轻盐胁迫伤害提供理论依据。结果显示:(1)NaCl胁迫显著抑制了番茄幼苗的生长、根系活力和SOD、POD、CAT活性,提高了电解质渗透率及MDA、Pro、可溶性糖含量;(2)外源喷施GSH能够诱导NaCl胁迫下番茄幼苗叶片抗氧化酶SOD、POD、CAT活性上调,电解质渗透率及MDA含量下降,Pro和可溶性糖含量恢复至对照水平;(3)外源喷施还原型谷胱甘肽抑制剂(BSO)使NaCl胁迫下番茄幼苗的根系活力以及抗氧化酶SOD、POD、CAT活性下降,脯氨酸含量提高;(4)喷施GSH可诱导BSO和NaCl共处理番茄植株的根系活力、SOD、POD、CAT活性提高,MDA和Pro含量降低。研究表明,外源GSH可通过提高促进盐胁迫下番茄幼苗植株渗透调节能力及清除活性氧的酶促系统的防御能力、降低细胞膜脂过氧化程度、保护膜结构的完整性,从而有效缓解NaCl胁迫对番茄幼苗生长的抑制,提高其耐盐性。     

一氧化氮和动脉粥样硬化

动脉粥样硬化是脂蛋白、单核细胞、巨噬细胞、T淋巴细胞与血管壁内皮细胞相互作用而导致的慢性炎症反应。这个炎症的过程由脂质浸润开始,涉及氧化应激反应,最终导致复杂的病理损伤和斑块的形成,斑块突出入血管,破裂形成血栓而导致急性的心肌梗塞或中风。激活内皮源性的一氧化氮合成酶而生成的一氧化氮（NO）能够预防动脉粥样硬化,并对不周发展阶段的动脉粥样硬化的病理形成均有改善和逆转作用。其生成的NO能抗氧化、清除自由基、抑制低密度脂蛋自在血管壁被氧化,防止氧化低密度脂蛋白（oxLDL）的产生,而影响脂质浸润;能抑制NFKB的激活和核内迁移,阻抑激活的内皮细胞表达黏附分子,减少嗜中性粒细胞和单核细胞的黏附和活化,减少血管壁的炎症反应;能抑制血小板黏附、聚集,抑制凝血酶诱导的血小板活性因子的表达以减少血栓形成;能阻止凋亡,保持内皮细胞的完整性;还能有效地抑制血管平滑肌细胞增殖、迁移和细胞外基质的合成,对动脉粥样硬化病理形成和发展具有阻抑作用。     

NO detection in biological samples: Differentiation of NO and NO using infrared laser spectroscopy

Accurate characterization of the biochemical pathways of nitric oxide (NO) is essential for investigations in the field of NO research. To analyze the different reaction pathways of enzymatic and non-enzymatic NO formation, determination of the source of NO is crucial. Measuring NO-related products in biological samples distinguishing between ¹⁴NO and ¹⁵NO offers the opportunity to specifically analyze NO signaling in blood and tissue. The aim of this study was to establish a highly sensitive technique for the specific measurement of NO in an isotopologue-selective manner in biological samples.With the cavity leak-out spectroscopy setup (CALOS) a differentiation between ¹⁴NO and ¹⁵NO is feasible. We describe here the employment of this method for measurements in biological samples. Certified gas mixtures of ¹⁴NO/N₂ and ¹⁵NO/N₂ were used to calibrate the system. and of aqueous and biological samples were reduced in a triiodide solution, and the NO released was detected via CALOS. Gas-phase chemiluminescence detection (CLD) was used for evaluation.The correlation received for both methods for the detection of NO in the gas phase was r = 0.999, p < 0.0001. Results obtained using aqueous and biological samples verified that CALOS enables NO measurements with high accuracy (detection limit for 0.3 pmol and 0.5 pmol; correlation ¹⁴NO: p < 0.0001, r = 0.975, ¹⁵NO: p < 0.0001, r = 0.969).The CALOS assay represents an extension of NO measurements in biological samples, allowing specific investigations of enzymatic and non-enzymatic NO formation and metabolism in a variety of samples.     

NO, NO, NO! Nitrosyl siblings from [IrCl5(NO)]

Pentachloronitrosyliridate(III) ([IrCl₅(NO)]⁻), the most electrophilic NO⁺ known to date, can be reduced chemically and/or electrochemically by one or two electrons to produce the NO and HNO/NO⁻ forms. The nitroxyl complex can be formed either by hydride attack to the NO⁺ in organic solvent, or by decomposition of iridium-coordinated nitrosothiols in aqueous solutions, while NO is produced electrochemically or by reduction of [IrCl₅(NO)]⁻ with H₂O₂. Both NO and HNO/NO⁻ complexes are stable under certain conditions but tend to labilize the trans chloride and even the cis ones after long periods of time. As expected, the NO⁺ is practically linear, although the IrNO moiety is affected by the counterions due to dramatic changes in the solid state arrangement. The other two nitrosyl redox states comprise bent structures.     

Differential cytostatic effects of NO donors and NO producing cells.

A 3-h exposure to NO donors (spermine-NO, DETA-NO, or SNAP), or to NOS II-expressing cells (activated macrophages or EMT6 cells) reversibly inhibited DNA synthesis in K562 tumor cells. In GSH-depleted K562 cells, cytostasis remained reversible when induced by DETA-NO or NOS II activity, but became irreversible after exposure to spermine-NO or SNAP. Only SNAP and spermine-NO efficiently inhibited GAPDH, an enzyme with a critical thiol, in GSH-depleted cells. Thus, the irreversible cytostasis induced in GSH-depleted cells by spermine-NO or SNAP can be tentatively attributed to S-nitrosating or oxidizing species derived from NO. However, these species did not contribute significantly to the early antiproliferative effects of macrophages. Ribonucleotide reductase, a key enzyme in DNA synthesis. has been shown to be inhibited by NO. Supplementation of the medium with deoxyribonucleosides to bypass RNR inhibition restored DNA synthesis in target cells exposed to DETA-NO and NO-producing cells, but was inefficient for GSH-depleted cells previously submitted to spermine-NO or SNAP. These cells also exhibited a persistent depletion of the dATP pool. In conclusion, GSH depletion reveals striking qualitative differences in the nature of the toxic effectors released by various NO sources, questioning the significance of S-nitrosating or oxidizing nitrogen oxides in NOS II-dependent cytostasis.     

Exchange of NO and NO2 between wheat canopy monoliths and the atmosphere

The fluxes of NO and NO₂ between wheat canopy monoliths and the atmosphere were investigated with the dynamic chamber technique. For this purpose monoliths were dug out at different plant growth stages from a field site, transported to the institute, and placed in an environmental growth chamber. The wheat canopy monoliths were exposed over a period of four days to the average ratios of atmospheric NO₂ and NO measured at the field site, i.e. NO₂ concentration of about 18 mL L^-1 plus NO concentration lower than 0.5 nL L^-1. Under these conditions NO emission into the atmosphere and NO₂ deposition into canopy monoliths was observed. Both fluxes showed diurnal variation with maximum rates during the light and minimum rates during darkness. NO₂ fluxes correlated with soil temperature as well as with light intensity. NO fluxes correlated with soil temperature but not with light intensity. From the investigation performed the diurnal variation of the NO and NO₂ compensation points, the maximum rates of NO and NO₂ emission, and the total resistances of NO and NO₂ fluxes were calculated. Under the assumption that the measured data are representative for the whole vegetation period, annual fluxes of NO and NO₂ were estimated. Annual NO emission into the atmosphere amounted to 87 mg N m^-2 y^-1 (0.87 kg ha^-1 y^-1), annual NO₂ deposition into canopy monoliths amounted to 1273 mg N m^-2 y^-1 (12.73 kg ha^-1 y^-1). Apparently, the uptake of atmospheric nitrogen by the wheat field from NO₂ deposition is about 15 times higher than the loss of nitrogen from NO emission. It can therefore be assumed that even in rural areas wheat fields are a considerable sink for atmospheric nitrogen. The annual sink strength estimated in the present study is ca. 12 kg N ha^-1 y^-1. The possible origin of the NO emitted and the fate of atmospheric NO₂ taken up by the wheat canopy monoliths are discussed.Preliminary results of this paper were presented at the Joint Workshop COST 611/Working Party 3 and EUROTRAC in Delft, The Netherlands (Ludwig et al., 1991).     

Heat-induced increases in endothelial NO synthase expression and activity and endothelial NO release

Endothelial nitric oxide (NO) synthase (eNOS) is regulated by heat shock protein 90 (HSP90), a heat-inducible protein; however, the effect of heat shock on eNOS expression and eNO release is unknown. Bovine aortic endothelial cells were incubated for 1 h at 37 degrees C, 42 degrees C, or 45 degrees C and cell lysates were evaluated with the use of Western blotting. We observed a 2.1 +/- 0.1-fold increase in eNOS protein content, but no change in HSP90 content, HSP70 content, or HSP90/eNOS association, 24 h after heat shock at 42 degrees C. We also observed a 7.7 +/- 1.5-fold increase in HSP70 protein content, but did not observe a change in eNOS or HSP90 24 h after heat shock at 45 degrees C. eNOS activity and maximal bradykinin-stimulated NO release was significantly increased 24 h after heat shock at 42 degrees C. Heat shock in rats (core temperature: 42 degrees C, 15 min) resulted in a significant increase in aortic eNOS, HSP90, and HSP70 protein content. The aorta from heat-shocked rats exhibited a decreased maximal contractile response to phenylephrine, which was abolished by preincubation with NG-nitro-l-arginine. We conclude that prior heat shock is a physical stimulus of increased eNOS expression and is associated with an increase in eNOS activity, agonist-stimulated NO release, and a decreased vasoconstrictor response.     

NO flowering

The complex control of flowering time ensures that plants flower in conditions favourable for reproductive success. A recent study adds another dimension to this established complexity by revealing that nitric oxide (NO) represses flowering in Arabidopsis. The analysis of recently identified mutants that either overproduce or are compromised in endogenous NO production has identified NO-sensitive features of the circuitry of flowering time control: NO acts to repress the amplification of gene expression dependent on the circadian clock and promotes the accumulation of mRNA encoding a key repressor of flowering, FLC.     

Ceruloplasmin is a NO oxidase and nitrite synthase that determines endocrine NO homeostasis

Nitrite represents a bioactive reservoir of nitric oxide (NO) that may modulate vasodilation, respiration and cytoprotection after ischemia-reperfusion injury. Although nitrite formation is thought to occur via reaction of NO with oxygen, this third-order reaction cannot compete kinetically with the reaction of NO with hemoglobin to form nitrate. Indeed, the formation of nitrite from NO in the blood is limited when plasma is substituted with physiological buffers, which suggests that plasma contains metal-based enzymatic pathways for nitrite synthesis. We therefore hypothesized that the multicopper oxidase, ceruloplasmin, could oxidize NO to NO+, with subsequent hydration to nitrite. Accordingly, plasma NO oxidase activity was decreased after ceruloplasmin immunodepletion, in ceruloplasmin knockout mice and in people with congenital aceruloplasminemia. Compared to controls, plasma nitrite concentrations were substantially reduced in ceruloplasmin knockout mice, which were more susceptible to liver infarction after ischemia and reperfusion. The extent of hepatocellular infarction normalized after nitrite repletion. These data suggest new functions for the multicopper oxidases in endocrine NO homeostasis and nitrite synthesis, and they support the hypothesis that physiological concentrations of nitrite contribute to hypoxic signaling and cytoprotection.     

Contribution of nNOS- and eNOS-derived NO to microvascular smooth muscle NO exposure.

Nitric oxide (NO) plays an important role in autocrine and paracrine manner in numerous physiological processes, including regulation of blood pressure and blood flow, platelet aggregation, and leukocyte adhesion. In vascular wall, most of the bioavailable NO is believed to derive from endothelial cell NO synthase (eNOS). Recently, neuronal NOS (nNOS) has been identified as a source of NO in the vicinity of microvessels and has been shown to participate in vascular function. Thus NO can be produced and transported to the vascular smooth muscle cells from 1). endothelial cells and 2). perivascular nerve fibers, mast cells, and other nNOS-containing sources. In this study, a mathematical model of NO diffusion-reaction in a cylindrical arteriolar segment was formulated. The model quantifies the relative contribution of these NO sources and the smooth muscle availability of NO in a tissue containing an arteriolar blood vessel. The results indicate that a source of NO derived through nNOS in the perivascular region can be a significant contributor to smooth muscle NO. Predicted smooth muscle NO concentrations are as high as 430 nM, which is consistent with reported experimental measurements ( approximately 400 nM). In addition, we used the model to analyze the smooth muscle NO availability in 1). eNOS and nNOS knockout experiments, 2). the presence of myoglobin, and 3). the presence of cell-free Hb, e.g., Hb-based oxygen carriers. The results show that NO release by nNOS would significantly affect available smooth muscle NO. Further experimental and theoretical studies are required to account for distribution of NOS isoforms and determine NO availability in vasculatures of different tissues.