大豆柑桔间作系统中磷的分配和迁移规律研究

用微区试验和³²P同位素示踪技术,比较研究了大豆、柑桔间作和单作条件下,P在大豆和柑桔体中的分配、转移及其在土壤中的迁移规律.结果表明,间作大豆的吸P量和各部位累积P量显著地低于单作大豆;³²P肥料浅施,间作大豆吸收的³²P量显著低于单作大豆;³²P肥料深施,间作大豆吸收的³²P量显著高于单作大豆,但间作不影响P和³²P在各部位的转移和分配.间作柑桔吸收的³²P量显著低于单作柑桔.柑桔新吸收的³²P可快速向地上部分输送,并优先供应生长活跃部位.间作不影响³²P在柑桔各部位的转移和分配,但是P肥深施使柑桔吸收的³²P向地上部分和生长活跃部位的转移速率减慢.间作使土壤中P的生物移动性增强,可促进土壤深层P向土壤浅层迁移.试验结果表明,大豆柑桔间作磷肥的施用深度以保持在20cm以内为佳.     

~(32)P示踪法研究溶磷真菌对磷肥转化固定和有效性的影响

采用³²P示踪技术,研究了溶磷青霉菌P8对肥料磷与土壤有效磷的转化、固定和有效性的影响.结果表明,溶磷青霉菌菌剂能够增加玉米、花生的生物量,促进作物对土壤和肥料磷素的吸收;溶磷菌剂具有防止有效磷转化为难溶Ca₁₀-P的作用,增加有效态磷(Ca₂-³²P、Ca₈-³²P)的比例.随时间延长,施入的³²P转化为Ca₁₀-P的数量(或比例)逐渐增加,但是相对于未接种菌剂处理,接种青霉菌菌剂的土壤磷和肥料磷转化为Ca₁₀-P比例最低.溶磷青霉菌菌剂不仅能够防止有效磷向难溶磷Ca₁₀-P的转化,而且其效果能够维持较长时间.     

温度对外源性32P在水、铜绿微囊藻和底泥中迁移的影响

采用同位素示踪法,在实验室模拟研究不同温度下外源性无机磷酸盐在水、铜绿微囊藻(Microcystis aeruginosa)和底泥中的迁移过程.外源性³²P加入水中后,首先是一种与温度无关的快速物理化学分配,大量溶解性磷酸盐迅速进入底泥和微囊藻中.随后水中³²P的迁移主要受微囊藻生长状况的影响.温度升高有利于微囊藻的生长,并提高了微囊藻吸磷的速度.微囊藻中最大外源性磷浓度只与水环境中的初始磷浓度有关.25℃时铜绿微囊藻的生长曲线有7d的对数期,没有明显的稳定期就转入衰亡期.在25℃时,当微囊藻超积累P到一定程度后,其对数生长同细胞内含P量无关.随着时间的推移,外源性³²P不断向底泥中迁移,实验末期所有的³²P都转移到底泥中.提高温度使水中溶解性外源性磷的下降速率加快,7d后水中溶解的外源性磷浓度低于0.00716mg·L^-1.     

三叶草体内磷通过菌丝桥向黑麦草的传递研究

应用5室分隔法研究了供体三叶草体内的³²P通过菌丝桥向受体黑麦草的传递作用。结果表明,菌根侵染供体三叶草根系之后,根外菌丝可穿过中室到达受体植株根室而再度侵染受体黑麦草的根系,从而形成三叶草-黑麦草根系之间的菌丝桥;供体三叶草体内的³²P可通过根间菌丝桥传递给受体黑麦草,³²P的传递量随受体植株施磷水平的提高而降低.     

不同浓度海水胁迫对菊芋幼苗生长发育及磷吸收的影响

种植抗盐耐海水植物是合理利用和开发海涂资源的有效措施之一。本试验通过不同浓度海水处理研究菊芋幼苗生长发育及对³²P吸收利用差异和离子吸收分布的情况。结果表明:在不同浓度海水浇灌下,菊芋地上部、地下部、总鲜重及干物质重从CK到50%海水浓度没有明显变化,在75%海水胁迫下显著下降,干物质百分比则为75%海水浇灌的最高;在中等P水平下,地上部在25%海水处理下对³²P吸收率最高;随海水浓度增高菊芋幼苗地上部单位干重积累的Na⁺和Cl^-依次增大;而K⁺与Na⁺积累情况不同,K⁺在25%海水胁迫下地上部单位干重积累的最多,其次是50%,CK和75%海水胁迫差不多;地下部单位干重积累的Na⁺、Cl^-和K⁺情况与地上部单位干重积累的各离子趋势相似。     

不同磷浓度对玉米生长及磷、锌吸收的影响

在不同磷水平(0.1、1.0、5.0、10和100μmol·L^-1P)的水培液中培养玉米苗,测定不同培养时期玉米的生长和玉米植株对P、Zn吸收和利用效率.结果表明,玉米在100μmol·L^-1P的溶液中生长速率最大,而根冠比在0.1μmol·L^-1P的溶液中为最大.随着水培液中P水平的增加,植株对P的吸收速率增加,而利用效率降低;玉米根系含Zn量增加,而冠层含Zn量变化不大,说明增P使Zn在根内富集,Zn向冠层转移速率较小,玉米幼苗根系中P和Zn的浓度呈正相关关系.     

硝酸盐供应水平对平邑甜茶幼苗生长、光合特性与15N吸收、利用的影响

以霍格兰营养液为培养基质,采用¹⁵N同位素示踪技术,研究不同浓度¹⁵NO₃^--N (0、2.5、5、10和20 mmol·L^-1,分别以N₀、N₁、N₂、N₃和N₄表示)对平邑甜茶幼苗生长、光合作用、¹⁵N吸收、利用及分配的影响.结果表明:与其他处理相比,N₂处理幼苗叶绿素含量、叶面积及各器官干质量最大.叶片净光合速率(P_n)随¹⁵NO₃^--N浓度的增加显著增大,但¹⁵NO₃^--N浓度超过N₂处理后P_n略有下降.处理20 d时,N₂处理幼苗根系活力最大,根系长度、根系总表面积和根尖数也显著高于其他处理.各处理间¹⁵N分配率差异显著,N₂处理幼苗各器官间¹⁵N分配率最均衡,¹⁵N利用率也较高;随¹⁵NO₃^--N浓度增加,各处理幼苗全氮量和¹⁵N吸收量呈先升高后降低的趋势,且在N₂处理时最大,分别为103.77和21.57 mg.处理12 d后,叶片硝酸还原酶(NR)活性以N₂处理最高,N₄处理最低,至第16天时,N₄处理较N₂处理降低了84.9%.因此,¹⁵NO₃^--N供应过低抑制幼苗光合作用及氮素吸收,¹⁵NO₃^--N供应过高则抑制幼苗体内硝态氮同化及根系生长,均不利于苹果幼苗生长及氮素营养吸收利用,适量供氮有利于苹果幼苗的生长、光合作用的提高,以及氮素的吸收、利用和分配.     

钨酸钠对苹果幼苗15N吸收利用、13C积累及果实品质的影响

分别以1年生苹果砧木M9T337幼苗和5年生烟富3/SH6/平邑甜茶为试材,开展盆栽和田间试验,并结合¹⁵N、¹³C同位素示踪技术,研究不同浓度(0、0.5、1、1.5 mmol·L^-1,分别用CK、T₁、T₂和T₃表示)硝酸还原酶(NR)抑制剂钨酸钠对苹果幼苗¹⁵N吸收利用、¹³C积累和成熟期果实品质的影响。结果表明: 盆栽试验中,喷施0.5~1.0 mmol·L^-1钨酸钠可显著抑制幼苗地上部生长,但对根系生长影响不显著;当钨酸钠浓度达到1.5 mmol·L^-1时可显著抑制根系生长。同一时期各处理叶片NR活性与钨酸钠浓度呈负相关,均表现为CK>T₁>T₂>T₃。随处理时间的延长,叶片硝态氮含量总体表现为先升高后降低的趋势,同一时期各处理硝态氮含量与钨酸钠浓度呈正相关,均表现为T₃>T₂>T₁>CK。喷施钨酸钠可不同程度地降低幼苗各器官¹⁵N吸收量和¹⁵N利用率,且钨酸钠浓度越高,抑制幼苗氮素吸收和利用的效果越显著。随钨酸钠浓度的提高,地上部¹³C积累量呈先升高后降低的趋势,在T₂处理时达到最高;幼苗整株¹³C积累量呈相似的规律。田间试验结果表明,喷施钨酸钠可降低成熟期叶片和果实的氮含量,果皮花青苷含量、果实可溶性固形物、可溶性糖含量和糖酸比均不同程度提高,其中T₂处理的效果最好。综上,T₂处理(1.0 mmol·L^-1钨酸钠)可有效抑制幼苗地上部生长,降低¹⁵N吸收利用,提高¹³C积累,有利于果实品质的提高。     

硝酸盐供应水平对平邑甜茶幼苗生长、光合特性与15N吸收、利用的影响

以霍格兰营养液为培养基质,采用¹⁵N同位素示踪技术,研究不同浓度¹⁵NO₃^--N (0、2.5、5、10和20 mmol·L^-1,分别以N₀、N₁、N₂、N₃和N₄表示)对平邑甜茶幼苗生长、光合作用、¹⁵N吸收、利用及分配的影响.结果表明:与其他处理相比,N₂处理幼苗叶绿素含量、叶面积及各器官干质量最大.叶片净光合速率(P_n)随¹⁵NO₃^--N浓度的增加显著增大,但¹⁵NO₃^--N浓度超过N₂处理后P_n略有下降.处理20 d时,N₂处理幼苗根系活力最大,根系长度、根系总表面积和根尖数也显著高于其他处理.各处理间¹⁵N分配率差异显著,N₂处理幼苗各器官间¹⁵N分配率最均衡,¹⁵N利用率也较高;随¹⁵NO₃^--N浓度增加,各处理幼苗全氮量和¹⁵N吸收量呈先升高后降低的趋势,且在N₂处理时最大,分别为103.77和21.57 mg.处理12 d后,叶片硝酸还原酶(NR)活性以N₂处理最高,N₄处理最低,至第16天时,N₄处理较N₂处理降低了84.9%.因此,¹⁵NO₃^--N供应过低抑制幼苗光合作用及氮素吸收,¹⁵NO₃^--N供应过高则抑制幼苗体内硝态氮同化及根系生长,均不利于苹果幼苗生长及氮素营养吸收利用,适量供氮有利于苹果幼苗的生长、光合作用的提高,以及氮素的吸收、利用和分配.     

等量分次施氮对冬枣15N和13C利用与分配特性的影响

以4年生盆栽冬枣为试材,采用¹³C、¹⁵N双标记示踪技术,在果实发育期研究了等氮量分次追施氮肥对冬枣植株¹⁵N和¹³C吸收、利用、积累和分配的影响.结果表明: 至果实采收期,冬枣各器官Ndff值(植株器官从肥料中吸收分配到的¹⁵N量对该器官全氮量的贡献率)随追氮次数的增多而显著增大.生殖器官(果实)和营养器官(叶片、枣吊、新生枣头枝和细根)的¹⁵N分配率以4次追氮处理最高,1次追氮处理最低,贮藏器官(主干、多年生枝和粗根)¹⁵N分配率的趋势相反;4次追氮处理¹⁵N利用率分别比1次和2次追氮处理高27.4%和15.5%.追氮次数越多,植株总氮量和¹⁵N吸收量越大;随时间的推移,1次追氮处理土壤¹⁵N丰度和总氮含量持续降低,2次追氮处理呈先升高后降低的趋势,4次追氮处理变化相对最为平稳,至处理后期显著高于其他处理;果实白熟至采收期,叶片叶绿素、氮含量和净光合速率均表现为4次追氮>2次追氮>1次追氮.不同处理¹³C同化物积累与分配不同.4次追氮处理¹³C固定总量分别是1次和2次追氮处理的1.1和1.2倍.增加追氮次数,促进了¹³C同化物向果实和贮藏器官的转移,而减少了向当年生营养器官的分配.综上,果实发育期4次追氮通过保证根层稳定、充足的氮素供应,提高了对氮素的吸收和利用,进而维持了较高的净光合速率,促进并优化了光合同化物的积累和分配,最有利于冬枣树体的生长及产量和品质的提高.     

Phosphorylation of an actin · tropomyosin · troponin complex from human skeletal muscle

A human skeletal actin · tropomyosin · troponin complex was phosphorylated in the presence of [γ-³²P]ATP, Mg²⁺, adenosine 3′:5′-monophosphate (cyclic AMP) and cyclic AMP-dependent protein kinase (protein kinase). Phosphorylation was not observed when the actin complex was incubated in the absence of protein kinase or 1 μM cyclic AMP. In the presence of 10⁻⁷ M Ca²⁺ and protein kinase 0.1 mole of [³²P]phosphate per 196 000 g of protein was incorporated. This was two-fold higher than the [³²P]phosphate content of a rabbit skeletal actin complex but two-fold lower than that of a bovine cardiac actin complex. At high Ca²⁺, 5 · 10⁻⁵ M, little change in the phosphorylation of a human skeletal actin complex occurred. Phosphoserine and phosphothreonine were identified in the [³²P]phosphorylated actin complex. Polyacrylamide gel electrophoresis in sodium dodecyl sulfate showed that 60% of the label was associated with the tropomyosin binding component of troponin. The inhibitory component of troponin contained 16% of the bound [³²P]phosphate. Increasing the Ca²⁺ concentration did not significantly decrease the [³²P]phosphate content of the phosphorylated proteins in the actin complex. No change in the distribution of phosphoserine or phosphothreonine was observed. Half maximal calcium activation of the ATPase activity of reconstituted human skeletal actomyosin made with the [³²P]phosphorylated human skeletal actin complex was the same as a reconstituted actomyosin made with an actin complex incubated in the absence of protein kinase at low or high Ca²⁺.     

Bradykinin effects on phospholipid metabolism and its relation to arachidonic acid turnovers in neuroblastoma × glioma hybrid cells (NG 108-15)

In neuroblastoma × glioma hybrid cells (NG 108-15) labelled with [³²P]-trisodium phosphate, [³H]-inositol and [¹⁴C]-arachidonic acid, bradykinin stimulated the hydrolysis of phosphatidylinositol 4,5-bisphosphate (PIP₂) while it had no effect on the release of [¹⁴C]-arachidonic acid (AA). The effect on PIP, was time- and dose-dependent with a maximal effect on [³H]-inositol- and [³²P]-labelled cells after 10–30 s of stimulation with 10⁻⁶ M bradykinin. However, the hydrolysis of [¹⁴C]-AA labelled PIP₂ was delayed compared to the effect on [³H]- and [¹⁴C]-PIP₂ and was not detectable until after 60 s of stimulation. Bradykinin stimulation resulted in an increased formation of [³H]-inositol phosphates (IP) and [³²P]- and [¹⁴P]- and [¹⁴C]-phosphatidic acid (PA) but the time course for PA formation did not allow the time-course for PIP₂ hydrolysis. A reduced labelling of [²³P]- and [¹⁴C]-phosphatidylcholine was also found in stimulated cells suggesting that PA may derive from other sources than PIP₂. In conclusion, our results indicate that bradykinin activates phospholipase C, but not phospholipase A₂, in NG 108-15 cells.     

Multi-site phosphorylation in ox-kidney branched-chain 2-oxoacid dehydrogenase complex

Tryptic [³²P]phosphopeptides were prepared from [³²P]phosphorylated ox-kidney branched-chain complex and analysed by high-voltage paper electrophoresis at pH 1.9. In the maximally phosphorylated complex 3 tryptic [³²P]phosphopeptides were identified (TA, TB, TC). R_F-values relative to N⁶-dinitrophenyllysine were (mean ± SEM for 25 obs.): TA, 1.53 ± 0.03; TB, 1.07 ± 0.02; TC, 0.65 ± 0.01. Relative rates of phosphorylation were TA> TB> TC. Phosphorylation of TA reached a maximum when about 66% of the complex was inactivated. Phosphorylation of TB and TC was associated mainly with 66–95% inactivation of the complex.     

The involvement of ecto-ATPase activity in the phosphorylation of intracellular proteins by the addition of extracellular [P]ATP in PC12 cells

We have investigated the possibility that ecto-phosphorylation by extracellular ATP may play a role in the development of PC12 cells. To test this model and to identify putative target membrane proteins, intact PC12 cells were radiolabeled by the addition of 20 μM [γ-³²P]ATP. An analysis of the labeled proteins revealed that a 57 kDa protein was the most abundant phosphorylated protein even within time periods as short as 3 min and continued to be labeled over and above the level of other proteins. This protein was identified as tyrosine hydroxylase by immunoprecipitation with antiserum to tyrosine hydroxylase. When intact cells were incubated with either [γ-³²P]ATP or ³²P_i of comparable specific radioactivity, the overall protein labeling pattern and the degree of phosphorylation of tyrosine hydroxylase were similar. There were no discrete proteins that were labeled by [γ-³²P]ATP and not by ³²P_i that would provide evidence for ecto-kinase activity in PC12 cells. Also, the addition of nonradioactive P_i reduced the incorporation of radioactivity into the protein from extracellular [γ-³²P]ATP. These results suggested that the phosphorylation of tyrosine hydroxylase by extracellular [γ-³²P]ATP required the initial hydrolysis of ATP and the subsequent incorporation of the ³²P_i into the intracellular ATP pool. To support this interpretation, we have demonstrated directly the presence of ecto-ATPase activity in intact PC12 cells by measuring the hydrolysis of extracellular [γ-³²P]ATP. Nearly 50% of the total ATP added (20 μM) was hydrolyzed within 10 min under conditions identical to those used to demonstrate intracellular protein phosphorylation. PC12 cells express both a Ca²⁺-dependent ecto-ATPase activity and a Mg²⁺-dependent ecto-ATPase activity. In addition, extracellular ATP is degraded enzymatically not only to ADP, but sequentially to adenosine. Our results also point out the difficulties inherent in attempts to identify ecto-kinase activity in cells that also contain ecto-ATPase activities.     

白浆土－植物系统营养物质转化机制及其有效性研究——Ⅰ．32P同位素示踪法对白浆土中P肥利用率

利用³²P同位素示踪法对白浆土中P肥利用率进行了研究.结果表明,在岗地白浆土上,表层土壤表现出一定程度的供P不足现象,白浆层土壤有效P含量严重缺乏.表层土壤中当季P肥利用率的变幅范围为6.09～12.35%,白浆层土壤P肥利用率为13%左右.施用有机肥能明显提高白浆土Olsen P的含量,加速土壤本身P的活化,各种有机物中,以猪粪对土壤潜在P的活化效果最好.将Olsen P与X值、A值比较,认为Olsen P是评价白浆上P肥力简便易行的可靠指标.     

Tumour-promoting phorbol esters inhibit agonist-induced phosphatidate formation and Ca flux in human platelets

Tumour-promoting phorbol esters (phorbol-12-myristate-13-acetate, PMA; phorbol-12,13-dibutyrate, PDBu) but not 4β-phorbol, activate protein kinase C. Using human platelets pre-labelled with quin2 or ³²PO₄ we examined the effects of these compounds on human platelet cytosolic free Ca²⁺ ([Ca²⁺]_j) and on [³²]phosphatidic acid ([³²P]PtdOH). PMA and PDBu, but not 4β-phorbol inhibited thrombin-, PAF- and vasopressin-induced elevation of [Ca²⁺], and [²⁺P]PtdOH formation. It is suggested that protein kinase C may act to terminate the transduction processes that link receptor occupancy to cellular activation.     

Triphosphorus pentaiodide (P3I5), a new phosphorus(III) halide

The novel phosphorus(III) halide I₂PP(I)PI₂ (P₃I₅) has been obtained in solution as one component of a complex reaction mixture by two different routes, and characterised by ³¹P NMR spectroscopy.