Zinc Chloride Methylene Blue, Ii. Preparation of Giesma and Wright Type Low Azure B Blood Stains from Dichromate Oxidized Commercial Dye

TO determine the amount of K₂Cr₂O₇ required to produce optimal Giemsa type staining, six 1 g amounts (corrected for dye content) of zinc methylene blue were oxidized with graded quantities of K₂Cr₂O₇ to produce 4, 8, 12, 16, 20 and 24% conversion of methylene blue to azure B. These were heated with a blank control 15 minutes at 100 C in 60-65 ml 0.4 N HCI. cooled, and adjusted to 50 ml to give 20 mg original dye/ml. Aliquots were then diluted to 1% and stains were made by the “Wet Giemsa” technic (Lillie and Donaldson 1979) using 6 ml 1% polychrome methylene blue, 4 ml 1% cosin (corrected for dye content), 2 ml 0.1 M pH 6.3 phosphate buffer, 5 ml acetone, and 23 ml distilled water. The main is added last and methanol fixed blood films are stained immediately for 20-40 min.

For methylene blue supplied by MCB 12-H-29, optimal stains were obtained with preparations containing 20 and 24% conversion of methylene blue to azure B. With methylene blue supplied by Aldrich (080787), 16% conversion of methylene blue to azure B was optimal. Eosinates prepared from a low azure B/methylene blue preparation selected in this way give good stains when used as a Wright stain in 0.3% methanol solution. However, when the 600 mg eosinate solution in glycerol methanol is supplemented with 160 mg of the same azure B/methylene blue chloride the mixture fails to perform well. The HCI precipitation of the chloride apparently produces the zinc methylene blue chloride salt which is poorly soluble in alcohol. It appears necessary to have a zinc-free azure B/methylene blue chloride to supplement the probably zinc-free eosinate used in the Giemsa mixture.     

A Chlorate-Formaldehyde Modification of the Golgi Method

Pieces of fresh nervous tissue 3-5 mm thick are put into a mixture of: 6% K₂Cr₂O₇, 40 ml; 5% KClO₃, 20 ml; 20% chloral hydrate, 30 ml; and concentrated formalin (38% HCHO), 10 ml; allowed to fix 3 days, with a daily change of fluid; transferred to 3% K₂Cr₂O₇ for 3 days, with twice daily changes; then to 1% AgNO₃ for 3 days at 20-25° C. Frozen sections are cut, dehydrated, cleared and mounted in Permount with a cover glass. The method gives good results for microglia and oligodendroglia in addition to the usual staining of nerve cells and their processes.     

The Presence of Lipids But Absence of Tannins in Elodea Idioblasts

The presence of tannins in the idioblasts of Elodea densa is conclusively disproved. Ten reagents for histochemical detection of tannin (K₂Cr₂O₇, K₃Fe(CN)₆, FeCl₃, (NH₄)₂MO₄, Nessler's reagent, Fehling's reagent, methylene blue, gelatin, iodine-KI and lead acetate) gave negative tests in Elodea idioblasts. Two reagents (1% aqueous caffeine and a saturated solution of Ca(OH)₂) gave apparently positive reactions that could be explained by the presence of lipids. Positive tests for lipids were obtained by direct microscopic examination of the removal of lipid materials from freeze-dried leaves, using a 1:1 ether-alcohol mixture. The lipid material was not removed when acetone was substituted for ether-alcohol. A lipoprotein complex was demonstrated by using Serra's method for masked lipids.     

Two new multi-cobalt-containing heteropolyoxotungstates

Two new multi-cobalt-containing polyoxotungstates K₄Na₆Co₂(H₂O)₁₂{Co(H₂O)₄[Co₂(H₂O)₁₀Co₄(H₂O)₂(B--SiW₉O₃₄)₂]₂} · 40H₂O (1) and K₁₀Na₂[Co₄(H₂O)₂(GeW₉O₃₄)₂] · 20H₂O (2) have been obtained by the routine synthetic reactions in aqueous solution. The polyoxoanion framework of 1 consists of two sandwich-type polyoxoanions [Co₄(H₂O)₂(B--SiW₉O₃₄)₂]¹²⁻ connected together by a [CoO₂(H₂O)₄] cluster to constitute the sandwich dimer, and then, four isolated Co(H₂O)₅ cations coordinate to the dimer through four μ₂-O atoms. The polyoxoanion 2 is isomorphic to the sandwich-type polyoxoanion [Co₄(H₂O)₂(B--SiW₉O₃₄)₂]¹²⁻ in 1. The magnetic property of compound 1 has been studied by measuring its magnetic susceptibility in the temperature range 2.0–300.0 K, indicating the existence of intramolecular ferromagnetic Co–Co interactions, and, the electrochemical properties of 1 and 2 are detected in the pH 4 buffer solution.     

茄子无土栽培氮磷钾浓度优化施肥方案

本试验采用三因子二次饱和D-最优设计(310),以蛭石为栽培介质,建立了以氮、磷、钾浓度为变量因子,茄子产量和品质为目标函数的三元二次数学模型,以期得到茄子优质高产最优氮磷钾浓度范围.对模型解析结果表明: 氮、磷、钾浓度对茄子产量和品质均有显著影响.对产量和品质的影响程度均以钾浓度较大,对产量的影响程度以氮浓度次之,磷浓度较小,对品质则为磷浓度次之,氮浓度较小.氮磷、氮钾、磷钾浓度交互对茄子产量均有显著影响;氮钾浓度交互对茄子品质亦有显著影响.在低水平条件下,茄子产量和品质均随氮、磷、钾浓度增加而增加,但超过一定范围后,茄子产量和品质均随之降低.通过计算机模拟运算得出,本试验条件下茄子单株产量达3600 g的施肥方案为:氮16.0～20.0 mmol·L^-1、磷2.2～2.6 mmol·L^-1、钾9.9～12.9 mmol·L^-1;品质综合评分在90分以上的施肥方案为:氮18.0～21.1 mmol·L^-1、磷1.9～2.6 mmol·L^-1、钾10.6～13.3 mmol·L^-1.试验小区茄子产量预期达到43.2 kg(6个月生长期)、品质综合评分高达90分以上的优质高产营养液氮磷钾浓度范围为:氮18.0～20.0 mmol·L^-1、磷2.2～2.6 mmol·L^-1、钾10.6～12.6 mmol·L^-1,适宜的N∶P₂O₅∶K₂O浓度比例约为1∶0.13∶0.62.     

Studies on Polychrome Methylene Blue III. Alkali Methods of Polychroming

Studies were made on the influence of time and temperature, of free access of air, of pH, of salt concentration, of evaporation and of various alkali salts as polychroming agents in the conversion of methylene blue into azures and other decomposition products. Extended spectrophotometric studies were made as a means of evaluating the rate of change and nature of final products, and staining tests were made as indicated.

Alkali polychroming of methylene blue proceeds equally well in the presence or absence of external oxygen. It is attended by a slow, continuous evolution of formaldehyde. It is accelerated by increase in concentration of alkali, by evaporation, by increase in pH, and by higher temperatures, but even the low pH levels and low alkali concentrations yield the same products if the process be continued long enough. This contrasts with the cessation of the polychroming on exhaustion of the oxidizing agent in the acid polychroming processes.

It is found that close control of pH, temperature, time, evaporation, access of air, and alkali concentration will enable the production on repeated trial of polychrome methylene blues which are spectroscopically and tinctorially closely similar. Nevertheless, spectroscopic control would appear to be indicated in manufacture.     

Sudan Black and Osmic Acid as Staining Agents for Testicular Interstitial Cells

Two standard cytological techniques have heen modified to stain specifically the interstitial cells of the testis. In Method 1, the tissue is fixed in Zenker-formol or Regaud's fluid for several hours or overnight and subsequently postchromed in 3% K₂Cr₂O₇ for 72 hr at 37°C. After paraffin embedding, sections are cut at 5μ, dewaxed, brought down to 70% alcohol and stained in an unfiltered saturated solution of Sudan black in 70% alcohol for 10-30 min. Sections are washed briefly in 70% alcohol to remove all excess dye, differentiated, if necessary, in 50% alcohol, downgraded to water and mounted in Farrants' medium or glycerol jelly. Interstitial cells: deep blue black; remainder of testicular tissue: light blue. Method 2 is essentially the Champy-Kull technique but specific staining for mitochondria is omitted and the sections are downgraded to water; then they are mounted in Farrants' medium or glycerol jelly without further treatment. In this way osmicated lipoids are preserved. Interstitial cells: conspicuous due to the variable number of black granules in their cytoplasm; the remainder of the tissue: yellow.     

安徽省冬小麦施肥现状与肥料利用效率

冬小麦是安徽省重要的粮食作物。合理施肥是冬小麦获得高产的重要措施,明确当前安徽省冬小麦施肥现状和存在的问题对于指导冬小麦科学施肥具有重要意义。本研究以安徽省冬小麦为对象,于2018年对全省冬小麦主产区1591户农户进行调查,调查内容包括肥料品种、肥料用量、施肥方式、种植面积和产量水平。根据调查结果统计分析安徽省冬小麦种植过程中的施肥现状及存在问题,并以全省冬小麦平均产量和平均施肥量为基准,采用Cate-Nelson方法(十字交叉法)评估安徽省冬小麦产量与氮、磷和钾肥施用的关系,以探索安徽省冬小麦进一步增产增效的主要施肥途径。结果表明: 安徽省冬小麦平均产量为5185 kg·hm^-2,氮、磷和钾肥平均施用量分别为206、80和78 kg·hm^-2。其中旱茬麦氮、磷和钾肥平均施用水平比稻茬麦分别高14、16和3 kg·hm^-2。总体上,安徽省冬小麦种植中化肥平均用量趋于合理化,但是在施肥方式、养分运筹和肥料品种上还存在不合理现象。Cate-Nelson方法结果表明,全省冬小麦氮、磷、钾肥施用量中,仅有23.8%、21.2%和25.7%低于全省平均水平却获得较高的产量,此时氮、磷、钾肥偏生产力最高;有26.3%、19.3%和22.5%的施用量低于全省平均水平但没有实现高产;有26.2%、29.6%和25.0%的施用量虽然获得了高产,但施用量较高,氮磷钾肥偏生产力较低。这说明安徽省冬小麦增产增效还有很大的空间。全省冬小麦基肥和追肥机械化比例分别为62.7%和10.0%。虽然氮肥普遍实现了分次施用,但氮肥作基肥的比例仍然占到全生育期氮肥总量的69.0%,应适当降低。此外,在肥料品种选择上存在偏施化肥、不重视有机肥等问题。     

A Rapid Silver-on-the-Slide Method for Nervous Tissue

A progressive silver staining method is described, which permits microscopic examination of the sections during the staining process. After formaldehyde fixation, dehydration and embedding in paraffin or celloidin, fine fibers and synaptic endings may be demonstrated. After formaldehyde fixation and mordanting in 3% K₂Cr₂O₇, myelinated fibers and mitochondria are specifically stained.

The unique feature of this method is, that the silver solution (0.5% protargol) is mixed with the reducing solution: 1.6% Rochelle salts, containing traces of Ag NO₃, MgSO₄, and K₂S (U.S.P.). The sections are placed directly into this mixture, which is then warmed to 45-55° C. Sections are removed when progressive staining is completed, washed in water, dehydrated and mounted.

In the fiber stain, nerve fibers and synaptic endings are dark brown or black, and nuclear chromatin is deep brown, against a pale yellow background. When the myelin sheath procedure is followed, the fiber bundles are deep brown, and the intensity of the staining remains the same for specific tracts, aiding in their identification.     

A Holocene environmental record from the southern Yangtze River delta, eastern China

The Holocene sedimentary record of core ZX-1, recovered west of mid-Holocene Chenier ridges on the monsoon-controlled Southern Yangtze delta, eastern China, consists of lagoon, salt marsh, upper tidal flat, and limnic facies, reflecting low-energy depositional environments. Holocene deposits mainly originated from the surrounding Tai Lake drainage basin. The temporal variation of most geochemical element percentages corresponds with the climatic phases inferred from the pollen record, i.e., the relatively low values of SiO₂, Na₂O, CaO and high values of Al₂O₃, K₂O, MgO, Fe₂O₃, FeO, FeO + Fe₂O₃ and TiO₂ generally concur with the warm and humid climate, and vice versa. Three geochemical indices − Al₂O₃/Na₂O, K₂O/Na₂O, and CaO/K₂O − are found to be sensitive to past precipitation in the monsoon-controlled southern Yangtze River delta. Based on fine sediment analysis of core ZX-1, the samples deposited under a dry climate with a mean annual precipitation (MAP) < 500–900 mm tend to have Al₂O₃/Na₂O values less than 12.2, and the samples deposited under a moist climate with an MAP 1000–1800 mm mostly have Al₂O₃/Na₂O values higher than 12.2. Similarly, the K₂O/Na₂O boundary value is 2.0. However, for CaO/K₂O, the dry climate sediments likely show values higher than 0.9, and those wet climate ones generally have values less than 0.9. This geochemical response suggests the potential application of these indices in the interpretation of palaeoclimate variation of monsoon-controlled eastern China.

Holocene climatic variation history is reconstructed for the southern Yangtze delta. From 8000 to 7000 yr BP, regional climate demonstrated frequent fluctuations, with warm and wet periods (8000–7700; 7500–7200 yr BP) alternating with cool and less humid periods (7700–7500; 7200–7000 yr BP). From 7000 to 6000 yr BP, the climate was relatively warm and humid. Since then, it had turned cool and dry, climaxing in an intense cold event around 4000 yr BP. After the cold event, it became warm and humid until around 2500 yr BP.     

Methylene Violet (Bernthsen), by Zinc-Alkali-Chlorate Hydrolysis of Methylene Blue

Though Bernthsen's methylene violet (MV) is a common constituent of polychrome methylene blue, the hydrolytic oxydation of methylene blue to yield azure-free MV has been considered a difficult chemical reaction since the time of Bernthsen, who used Ag₂O in the hydrolysis. MV is qualitatively distinguished from azures by Bernthsen's criteria and the author's new tests: (1) light-excited isomeric change, (2) reactivity to acidity, (3) reaction with KCIO, and (4) reaction with Na₂SO₃ of azures in CHCI₃, while MV gives none. But MV shows (5) indicator properties at pH 4, while azures do not. For practical hydrolysis, treat methylene blue (10 parts by weight) and KCIO₃ (1 part) with 1-2 N NaOH to convert methylene blue to a mixture of MV and azures. Then dilute the solution, add a Zn salt and NaHCO₃ in excess of the amount needed to convert the NaOH to Na₂CO₃. Boil the solution gently for 1-2 hr. The end point of the reaction is found by pipetting a drop of reactant into 3% acetic acid in a test tube, adding CHC1₃ and extracting. The acetic layer should then be almost colorless while the CHC1₃ is colored intensely cherry red. After cooling, the precipitated dye is filtered and dried. This procedure gives good yields of a dye which meets the criteria given by Bernhsen. The peak of the absorption curve in solution, pH 4-11, is at 624 mμ (Bernthsen 625 mμ) and in acid solution, pH 0-4, 588 mμ (Biological Stains, 1953; 580 μ). The dye contains so little azures, that purification of the MV fraction obtained from the reaction mixture is unnecessary when it is used in the Wright-type Romanowsky stain. The remarkable staining effect of MV is its power to bring out red azurophil granules of monocytes and lymphocytes when used with eosinated thiazins in Wright's stain.     

Studies of the oxovanadium(IV)—oxalate system: syntheses and crystal structures of binuclear (Ph4P)2[(VO)2(H2O)2(C2O4)3]·4H2O and of the one-dimensional chain material, (Ph4P)[VOCl(C2O4)]

The hydrothermal reactions of (Ph₄P)[VO₂Cl₂] and H₂C₂O₄ at 150 and 125°C yield (Ph₄P)₂[V₂O₂(H₂O)₂(C₂O₄)₃]·4H₂O (1) and (Ph₄P)[VOCl(C₂O₄)] (2), respectively. The structure of the molecular anion of 1 consists of a binuclear unit of oxovanadium(IV) octahedra bridged by a bisbidentate oxalate group. The VO₆ coordination geometry at each vanadium site is defined by a terminal oxo group, an aquo ligand, and four oxygen donors — two from the bisbidentate bridging oxalate and two from the terminal bidentate oxalate. The structure of 2 consists of discrete Ph₄P⁺ cations occupying regions between [VOCl(C₂O₄)]⁻_∞ spiral chains. The structure of the one-dimensional anionic chain exhibits V(IV) octahedra bridged by bisbidentate oxalate groups. Crystal data: 1·4H₂O, monoclinic P2₁/n, A = 12.694(3), B = 12.531(3), C = 17.17(3) Å, β = 106.32(2)°, V = 2621.3(13) ų, Z = 2, D_calc = 1.501 g cm⁻³, structure solution and refinement converged at a conventional residual of 0.0518; 2, tetragonal P4₃, A = 12.145(2), C = 15.991(3) Å, V = 2358.7(12) ų, Z = 4, R = 0.0452.     

Structural determinations, magnetic and EPR studies of complexes involving the Cr(OH)2Cr unit

Five heterometallic compounds with formulae [Ba(H₂O)₄Cr₂(μ-OH)₂(nta)₂] · 3H₂O (I), [M(bpy)₂(H₂O)₂] [Cr₂(OH)₂(nta)₂] · 7H₂O, where M²⁺ = Zn, (II); Ni, (III); Co, (IV) and [Mn(H₂O)₃(bpy)Cr₂(OH)₂(nta)₂] · (bpy) · 5H₂O (V); bpy = 2,2′-bipyridine, (nta = nitrilotriacetate ion) have been prepared by reaction of I with the corresponding M^II-sulfates in the presence of 2,2′-bipyridine. Substances I–V have been characterized by magnetic susceptibility measurements, EPR and X-ray determinations. I represents a 2D coordination polymer formed by coordination of centrosymmetrical dimeric chromium(III) units and Barium cations. The 10-coordinate Ba polyhedron is completed by four water molecules. Compounds II–IV are isostructural and consist of non-centrosymmetric dimeric anions [Cr₂(μ-OH)₂(nta)₂]²⁻, complex cations [M^II(bpy)₂(H₂O)₂]²⁺ and solvate water molecules. The octahedral coordination of chromium atoms implies four donor atoms of the nta³⁻ ligands and two bridging OH groups. Multiple hydrogen bonds of coordinated and solvate water molecules link anions and cations in a 3D network. A similar [Cr₂(μ-OH)₂(nta)₂]²⁻ unit is found in V. The bridging function is performed by a carboxylate oxygen atom of the nta ligand that leads to the formation of a trinuclear complex [Mn(bpy)(H₂O)₂Cr₂(μ-OH)₂(nta)₂]. Experimental and calculated frequency and temperature dependences of EPR spectra of these compounds are presented. The fine structure appearing on the EPR spectra of compound V is analyzed in detail at different temperatures. It is established that the main part of the EPR signals is due to the transitions in the spin states of a spin multiplet with S = 2. Analyses of experimental and calculated spectra confirm the absence of interaction between metal ions (M^II) and Cr-dimers in complexes III and IV and the presence of weak Mn–Cr interactions in V. The temperature dependence of magnetic susceptibilities for I–V was fitted on the basis of the expression derived from isotropic Hamiltonian including a bi-quadratic exchange term.     

A Glutaraldehyde-Dichromate-Silver Sequence for Differentiating Norepinephrine Cells from Epinephrine Cells in Neonatal and Adult Rats—Paraffin Sections

A glutaraldehyde-K₂Cr₂O₇ procedure intensified by silver staining enabled norepinephrine and epinephrine cells to be distinguished readily in paraffin sections of the adrenal glands of rats 8 days after birth. The technique involved fixation in 0.1 M cacodylate-buffered 5% glutaraldehyde (6-24 hr), treatment with 3.5% K₂Cr₂O₇ (6-12 hr) and routine preparation of paraffin sections. The sections were deparaffinised, brought to water and immersed in Fontana's solution (24 hr), prepared by adding concentrated NH₄OH drop by drop to 5% AgNO₃ until the precipitate formed just redissolved; more 5% AgNO₃ was then added until a permanent cloudiness just developed. After a rinse in distilled water, the sections were treated with 0.5% gold chloride (5 min) and Na₂S₂O₃ (5 min), then mounted in Depex. This sequence resulted in an intense black cytoplasmic colouration in norpinephrine-containing cells of both the adult and 8-day-old animals whereas epinephrine-containing cells remained colourless. The glutaraldehyde-K₂CrO₇ procedure, without intensification, gave very clear results in the adult: a yellow cytoplasmic colour in the norepinephrine cells with epinephrine cells colourless. A glutaraldehyde-OsO₄ sequence gave a less well defined separation of these cell types in the adult and failed to distinguish the cell types in the neonate.     

A Copper Sulfate-Silver Nitrate Method for Nerve Fibers of Planarians

For staining in toto, planarians are fixed in a mixture of 10 ml of commercial formalin, 45 ml of 95% ethanol and 2 ml of glacial acetic acid. After treatment with 70% ethanol 3-10 days, they are washed in distilled water and immersed in 10% CuSO₄. 5H₂O for 3 hr at 50° C, transferred without washing to 1% AgNO₃ for 1.0-1.5 hr at 50° C; and then developed in: 10 ml of 1% pyrogallol, 100 ml of 56% ethanol and 1 ml of 0.2% nitric acid. Gold toning, 5% Na₂S₂O₃ and dehydration follow as usual. For staining sections, material is fixed in the same fixative, embedded in paraffin and sectioned at 10 μ. After bringing sections to water, they are immersed in 20% CuSO₄. 5H₂O for 48 hr at 37° C; then rinsed briefly in distilled water and placed in 7% AgNO₃ for 24 hr at 37° C. They are washed briefly in distilled water and reduced in: hydroquincne, 1 gm; Na₂SO₃, 5 gm and distilled water 100 ml. Gold toning, followed by 5% Na₂S₂O₃ and dehydration completes the process. Any counterstaining may follow.     

Myelin Impregnation: An Improved Golgi-Cox Modification

Optic tecta of goldfish were coated with egg yolk and immersed for only one week in one of the following impregnation fluids: a) Solution A + B; A = 1 g K₂Cr₂O₇ and 1 g HgCl₂ boiled for 15 min in 85 ml distilled water and allowed to cool; B = 0.8 g K₂Cr₂O₇ and 0.5 g KWO₄ dissolved in 20 ml distilled water, b) Solution A + B two volumes diluted with boiled distilled water, c) Solution A + B four volumes diluted with boiled distilled water. Each tectum was immersed 6 hr in 100 ml distilled water containing 0.5 g LiOH and 15 g KNO₃, washed 18 hr in 500 ml 0.2% acetic acid, dehydrated with ethanol, and embedded in low viscosity nitro cellulose. Sections were cut at 100 pm with a rotary microtome after clearing with cedarwood oil. Methods b) and c) have two advantages compared with method a), the original Golgi-Cox method. First, more cells are impregnated, especially in the layers extending 200-400 μm below the surface, and dendrites as well as unmyelinated axons are well impregnated. Second, myelin sheaths are impregnated and can be recognized by their peculiar chain-like appearance. The described Golgi-Cox modification offers an appropriate method to study the morphology of superficially located nervous tissue.     

Influence of different site symmetries of Eu centers on the luminescence properties of Anderson-based compounds

Two compounds, [Eu(H₂O)₇][Al(OH)₆Mo₆O₁₈] · 4H₂O (1) and {(C₂H₅NO₂)₂[Eu(H₂O)₅]}[Al(OH)₆Mo₆O₁₈] · 10H₂O (2), have been synthesized by conventional solution method and determined by single-crystal X-ray diffraction. Compound 1 shows a 1D chain structure built up of alternating Anderson-type polyanions [Al(OH)₆Mo₆O₁₈]³⁻ and hydrated rare-earth ions Eu³⁺. Compound 2 displays a 3D supramolecular network structure containing 1D sandglass-like channels along c axis, which were occupied by repetitive array of (H₂O)₈ clusters. Extensive hydrogen bonds play an important role in the formation of the 3D structures of 1 and 2. Luminescence measurements reveal that 1 and 2 exhibit intense red and orange fluorescent emission at room temperature, respectively. Origin of the distinct emission can be assigned to the different site symmetries of Eu³⁺ centers in the two compounds. These results are consistent with the crystal structures of the two compounds.     

Staining of Mitochondria with Aniline-Acid Fuchsin After Zenker-Formol Fixation

It was observed that mitochondria are well-demonstrated by aniline-acid fuchsin staining after Zenker-formol fixation if the sections are not de-Zenkerized. Tests showed that after mordanting in HgCl₂, K₂Cr₂O₇, FeCl₃, or FeSO₄, mitochondria in sections from tissues fixed in neutral buffered formalin could be stained fairly intensely by the same method. Salts of Ag, Ba, Ca, Cd, Co, Cu, Mg, Mn, and Zn were ineffective. If the presence of occasional mercury crystals in the sections is not objectionable, demonstration of mitochondria in Zenkerformol fixed tissues offer speed and additional flexibility in the subsequent use of the blocks as advantages over usual methods.     

N,N′-Ethylene-bis(3-methoxysalicylideneimine) mononuclear (4f) and heterodinuclear (3d–4f) metal complexes: Synthesis, crystal structure and luminescent properties

The stepwise synthesis of mononuclear (4f) and heterodinuclear (3d–4f) Salen-like complexes has been investigated through structural determination of the intermediate and final products occurring in the process. In the first step, reactions of ligand H₂L and Ln(NO₃)₃ · 6H₂O give rise to three mononuclear lanthanide complexes Ln(H₂L)(NO₃)₃ [H₂L = N,N′-ethylene-bis(3-methoxysalicylideneimine), Ln = Nd (1), Eu (2) and Tb (3)], in which N,N′-ethylene-bis(3-methoxysalicylideneimine) acts as tetradentate ligands with the O₂O₂ set of donor atoms capable of effective coordination. These species are fairly stable and have been isolated. Then, addition of Cu(Ac)₂ · H₂O to the mononuclear lanthanide complex yields expected heterodinuclear (3d–4f) complexes Cu(L)Ln(NO₃)₃ · H₂O [Ln = Nd (4) and Eu (5)] where the Cu(II) ion is inserted to the inner N₂O₂ cavity. Luminescent analysis reveals that complex 3 exhibits characteristic metal-centered fluorescence of Tb(III) ion. However, the characteristic luminescence of both Sm(III) and Eu(III) ions is not observed both in solution and solid state of the complexes.     

Staining Tissue of the Central Nervous System with Luxol Fast Blue and Neutral Red

The tissue is fixed in 10% neutral saline formalin for 1 day to 3 wk depending on the size of the block, dehydrated and embedded in paraffin. The sections are stained at 57° C for 2 hr, then at 22° C for 30 min, in a 0.0125% solution of Luxol fast blue in 95% alcohol acidified by 0.1% acetic acid. They are differentiated in a solution consisting of: Li₂CO₃, 5.0 gm; LiOH-H₂O, 0.01 gm; and distilled water, 1 liter at 0-1° C, followed by 70% alcohol, and then treated with 0.2% NaHSO₃. They are soaked 1 min in an acetic acid-sodium acetate buffer 0.1 N, pH 5.6, then stained with 0.03% buffered aqueous neutral red. Sections are washed in distilled water, 1 sec, then treated with the following solution: CuSO₄·5H₂O, 0.5 gm; CrK(SO₄)₂·12H₂O, 0.5 gm; 10% acetic acid, 3 ml; and distilled water, 250 ml. Dehydration, clearing and covering complete the process. Myelin sheaths are stained bright blue; meninges and the adventitia of blood vessels are blue; red blood cells are green. Nissl material is stained brilliant red; axon hillocks, axis cylinders, ependyma, nuclei and some cytoplasm of neuroglia, media and endothelium of blood vessels are pink.