Mercuric Bromphenol Blue Staining of Precipitin Lines in Agar

Lines formed by antibody-organ antigen reactions are stained particularly well by a modification utilizing the mercuric bromphenol blue (MBB) mixture of Mazia et al. (Biol. Bull., 104: 57-67, 1953). The agar covered slides are placed overnight in 0.85% NaCI at 4 C, followed by washing for 2 hr in 0.85% NaCI at 25 C. They are then rinsed for 10 min in distilled water, and dried overnight at 37 C. The precipitin lines are fixed by immersing the slides for 25 min in 95% alcohol, followed by 5 min hydration in distilled water. They are stained for 25 min in MBB mixture (HgCI₂, 10 gm; bromphenol blue, 0.1 gm; 95% ethanol, 100 ml). Excess stain is removed by immersing in acidified alcohol (95% ethanol, 98 ml; glacial acetic acid, 2 ml). Finally, the slides are passed through alcohol and xylene, and resin-mounted under coverslips.     

A Pollen Grain Squash Technique for Saccharum and Related Genera

Anthers collected between 9 and 10 AM were treated for 1 hr at 26-28 C with a 0.5% solution of colchicine, washed for 2-4 min in water, placed in 0.002 M 8-hydroxyquinoline for 1 hr, washed in water for 10 min and fixed in: methanol, 60 ml; chloroform, 30 ml; distilled water, 20 ml; picric acid, 1 gm and mercuric chloride 1 gm, for 24 hr. After washing they were hydrolysed in 1 N HCl for 15 min at 60 C, stained in leuco basic fuchsin for 30 min, then smeared on a slide in a drop of acetocarmine. The slides were sealed, stored overnight, the paraffin was removed, and the slide passed through a 1:1 mixture of n-butyl alcohol and acetic acid, then through pure n-butyl alcohol and mounted in Canada balsam. The significant features of this procedure are: (1) use of chromosomes in the haploid condition for karyotype analysis, (2) better exaggeration of constrictions for easier interpretation of chromosome types and (3) good spreading in plants with a large chromosome number.     

An Acetic Acid Dissociation, Air-Drying Technique for Insect Chromosomes, With Aceto-Lactic Orcein Staining

The method differs from mammalian techniques for somatic chromosomes in that it uses very small amounts of material. Drosophila melanogaster and an ant, Dorymyrmex sp., are used as examples. Pretreatment with 0.05% Colcemid in insect Ringer solution is applied to mature Drosophila larvae for 5 hr, by feeding, but Dorymyrmex prepupae require puncture and a 15 hr exposure of the puncture to the solution. Organs are removed under 1% sodium citrate, tansferred to fresh citrate for 10-20 min, than fixed in acetic-methanol, 1:3, for 30 min. Transfer to a drop of 60% acetic acid on a clean warmed slide dissociates the cells, which are spread by adding a small drop of fixative and tilting the slide in all directions. After immersion in acetic ethanol, 1:3, for 4 hr, rinsing in the stain solvent and draining the slides then have 2-3 drops of aceto-lactic orcein placed on each, coverslips added, and warmed (at about 50 C) for about 12 hr or until staining is sufficient. They can then either be treated as semipermanent or made permanent by allowing the coverslips to slide off in acetic-ethanol, dehydrating, and mounting in Euparal, or a synthetic resin.     

Enhanced Differentiation of Zaprionus Chromosomes by Prestaining Acid Hydrolysis

Two variations of orcein staining have been adapted to salivary gland chromosomes of Zaprionus. Method I: after dissection, glands are transferred to 1 N HCl at 60° C for 5 min, stained with 2.5% orcein in 60% acetic add for 15-20 min, and squashed in 60% acetic acid. Method II: after dissection, glands are transferred to 1 N HCl at 60° C for 5 min, transferred to a saturated solution of carmine in 45% acetic acid for 1 min, then to a mixture of 50 ml of 1% orcein in concentrated lactic acid and 50 ml of 30% acetic add for 5 min. They are squashed in the same mixture. The unproved differentiation of chromosomes from cytoplasm is attributed to the removal of cytoplasmic ribonucleic add by add hydrolysis.     

Simultaneous Formalin Fixation and Edta Decalcification, With Carbowax Embedding for Preservation of Acid Phosphatase

Carbowax serial sections from pubic symphyses of female mice, fixed and decalcified in a 10% formalin-5% Versenate solution for 18 hr at 4 C, pH 5.2, were incubated for 30 min with Burstone's simultaneous coupling reagent (pH 5.2); substrate: naphthol AS-TR and the diazonium salt, fast red violet L.B. All sections were counterstained with 1% methyl green at pH 4.0 in a phospho-citrate buffer. Inhibition by 0.01 M NaF, 0.0002 M CuCl₂, 10% tartaric acid and 0.01 M NaCN, as well as substrate-deficient and heat-inactivated controls, demonstrated conclusively that acid phosphatase was functionally preserved. Strong enzymatic activity was exhibited by osteoclasts, chondroclasts and free multinucleated giant cells. In addition, megakaryocytes, histiocytes, plasma cells, and monocytes exhibited moderate activity. The results demonstrated the technique to be consistently reproducible.     

Biosynthesis and properties of an extracellular metalloprotease from the Antarctic marine bacterium Sphingomonas paucimobilis

An extracellular protease from the marine bacterium Sphingomonas paucimobilis, strain 116, isolated from the stomach of Antarctic krill, Euphausia superba Dana, was purified and characterized. The excretion of protease was maximal at temperatures from 5 to 10°C, i.e. below the temperature optimum for the strain growth (15°C). The highly purified enzyme was a metalloprotease [sensivity to ethylenediaminetetraacetic acid (EDTA)] and showed maximal activity against proteins at 20–30°C and pH 6.5–7.0, and towards N-benzoyl-tyrosine ethyl ester (BzTyrOEt) at pH 8.0. At 0°C the enzyme retained as much as 47% of maximal activity in hydrolysis of urea denatured haemoglobin (Hb) (at pH 7.0), and at −5 and −10°C, 37 and 30%, respectively. The metalloprotease was stable up to 30°C for 15 min and up to 20°C for 60 min. These results indicate that the proteinase from S. paucimobilis 116 is a cold-adapted enzyme.     

An Arginine Histochemical Method Using Sakaguchi's New Reagent

A mounted paraffin section of material fixed in Bouin's, Carnoy's or 10% formalin is allowed to stand 15 minutes at room temperature in a 0.3% solution of 8-hydroxyquinoline in 30% ethanol. The slide, with adhering solution, is placed in 0.15 N hypochlorite (with enough KOH added to make the solution 0.015 N KOH) for 60 seconds, then (without draining) into a solution containing: 10 ml. of 0.15 N KOH; 15 g. of urea; 70 ml. of tertiary butyl alcohol, and water to make 100 ml. Here it is gently agitated for 10 sec. and then kept in a second change of the same solution for 2 min. Two changes of pure tertiary butyl alcohol, 10 sec. and 4 min.; one in aniline, 3 min.; and one of 10 sec. in xylene, complete the procedure. Permount containing 0.02% aniline is used as a mounting medium.     

Histochemical Demonstration of Succinic Dehydrogenase in Ascites Tumor Cells

Fresh undiluted tumor ascites (0.05 ml) withdrawn from peritoneal cavity was placed immediately in a centrifuge tube containing 2.0 ml of an aqueous mixture prepared with 1 part each of the following solutions: 1% neotetrazolium chloride, 0.2 M sodium succinate and 0.1 M phosphate buffer, pH 7.4. The tube was incubated for 2 hr at 37°C and centrifuged for 3 min at 700 rev/min. The precipitate was washed with 0.85% saline solution and subsequently fixed with neutral 10% formalin for 10 min. After centrifugation, smears or squash preparations of the precipitate were prepared. Succinic dehydrogenase activity was demonstrated very distinctly and uniformly by the granular deposition of a deep purple pigment intracellularly.     

Water-Pretreatment Squash Technic: A New and Simple Practical Method for the Chromosome Study of Animals

To simplify the staining of animal chromosomes (especially in insect testes) the authors have borrowed (with necessary modifications) the squash technic of plant cytology. The method has four steps: (1) Water pretreatment. This step requires only about 5-10 minutes either in water at room temperature or in water kept at about 38°C. in a water bath. (2) Fixation. Ordinarily only 5 minutes in 10-15% aqueous solution of glacial acetic acid is necessary. (3) Staining. The fixed tissue is rinsed in two or three changes of distilled water and then placed in a solution of basic fuchsin: either 1% in 30% ethyl alcohol, or 0.2-0.4% in 5-10% lactic acid. In the former solution the staining period should be about 2 minutes: in the latter, 5-20 minutes. The time is not critical. (4) Squashing. The material is rinsed in several changes of distilled water, placed on a clean slide and squashed under a cover glass. Such preparations last 4-5 weeks, and a technic is described for removing the cover glass in order to mount in Euparal and to make them permanent. The authors list various species of vertebrates as well as invertebrates in which the technic has given good chromosome staining, as shown by illustrations.     

Glutaraldehyde-Ammoniacal Silver Carbonate-Formaldehyde Staining of Histones of Mitotic Chromosomes

Cells from monolayer culture of Chinese hamster line Don were treated by Colcemid (0.1 μg/ml) for 2 hr, trypsinized and spun; resuspended in 0.5% sodium citrate solution for 10 min, respun, and then resuspended in a small volume of the supernatant. Slide preparations were made by smearing, followed by air drying for 1 min at room temperature. They were fixed and stained by the following sequence: 2.5% glutaraldehyde in Millonig's buffer, 30 min; distilled water, 6 min, 5 changes; ammoniacal silver at 18-26 C, 10 sec; distilled water, 30 min, 5 changes; 2.5% formalin, 2 min; and distilled water, 3 changes during 15 min. Staining solution: add 225 ml of 5% Na₂CO₃ to 75 ml of 10% AgNO₃, then add concentrated NH₄OH slowly, drop by drop, until the solution is transparent. Finally add 300 ml of dstilled water. Cells treated with cold 0.25 N HCl before fixation were not stained. Sequence modifications show that chromatin does not reduce silver by itself. This method stains the sites of high histone concentrations in mitotic chromosomes of cytogenetic preparations.     

雪腐核盘菌菌核的萌发条件与致死温度

菌核是核盘菌Sclerotinia spp.在土壤中的主要存活形式和菌核病的主要初侵染源,在土壤中可存活8年以上,其数量和存活状况直接影响着菌核病的发生和危害程度.本研究以雪腐核盘菌Sclerotinia nivalis菌株SS-TB为材料,分析了菌核萌发的影响因素、致死温度以及土壤温度对菌核存活的影响.结果 表明,未...     

Double Staining of Plant Materials in Bulk

Ovaries and ovules of Oryza sativa and Zea mays were collected between 9-30 and 10-30 AM, fixed in formalin-acetic-alcohol, stained in Delafield's hematoxylin for 2-4 hr, dehydrated through graded ethanol, counterstained for 3-4 hr either in light green, orange G or fast green (0.05-0.1%) at the 1:1 alcohol-xylene stage and embedded. A few ovaries were hydrolysed in 1 N HCI for 25 min at 60 C, stained in leuco basic fuchsin for 60-90 min, rinsed 3 times with a mixture of: 10% Na₂S₂O₅, 1; N HC1, 1; and distilled water, 18; washed repeatedly in distilled water, dehydrated through graded ethanol, counter-stained for 3-4 hr either with light or fast green (0.05-0.1%) at the 1:1 alcohol-xylene stage and embedded. Microtome sections were cut, ribbons mounted, dried, paraffin removed with xylene, and mounted in balsam. Uniformly stained preparations resulted and the dilute stains gave vivid color contrasts. Large numbers of ovules and ovaries can be processed in a short time, and reliable percentages of viable embryo sacs in normal, sterile and semisterile plants obtained.     

Hematoxylin-Eosin Staining of OsO4-Fixed Epon- Embedded Tissue; Prestaining Oxidation by Acidified H2O2

Successful application of hematoxylin-eosin staining to 0.5-1 μ sections of OsO₄-fixed Epon-embedded mammalian tissue is made possible by first treating the sections for approximately 1 min at 25-30 C with 10% H₂O₂ acidified with 0.1 or 0.01 N H₂SO₄ to pH 3.2. Subsequent steps are: washing; drying; Hams hematoxylin at 50 C, 1-2 min; washing; drying; 0.2-0.3% NH₄OH in 70% ethanol, 3-5 sec, drying at 50 C; 5% aqueous eosin for 3 & 45 sec at 25-30 C, washing; drying; clearing in xylene and mounting in resin. The use of acidified H₂O₂ prevents the staining of Epon and permits the characteristic staining picture to be obtained. Sections were attached to glass slides without adhesive and processed horizontally on a rack. Slides should be well drained and blotted before each drying step, to prevent formation of precipitate on the section.     

Use of Gallocyanin as a Myelin Stain for Brain and Spinal Cord

Tissue fixed in 10% formalin, formol saline, CaCO₃ or phosphate buffer neutralized formalin, Baker's formol calcium, Cajal's formol ammonium bromide, formalin-95% ethanol 1:9, formalin-methanol 1:9, Lillie's methanol-chloroform or Salthouse's formol cetyltrimethylammonium bromide was dehydrated and embedded in paraffin. Sections were attached to slides with either albumen or gelatine adhesive and processed throughout at room temperature of 22-25 C. Mordanting 30-60 min in 1% iron alum was followed by a 10 min wash in 4 changes of distilled water. Myelin was stained in a gallocyanin self-differentiating solution for 1-2.5 hr; thick sections requiring the longer time. The staining solution (pH approximately 7.4) consisted of Na₂CO₃, 90 mg; distilled water, 100 ml; gallocyanin, 250 mg; and ethanol, 5 ml. The ethanol was added to this mixture last, and after the other ingredients had been boiled and then cooled to room temperature. After a staining and thorough washing, Nissl granules were stained for 5-10 min in a solution consisting of: 0.1 M acetic acid, 60 ml; 0.1 M sodium acetate, 40 ml; methyl green, 500 mg. Washing, dehydration, clearing and mounting completed the process. Myelin sheaths were stained dark violet; neuronal nuclei, light green with dark granules of chromatin; nucleoli of motor cells and erythrocytes, dark violet; cytoplasm, green with dark green Nissl granules. The simple and reliable method can be adapted easily for use with automatic tissue processors.     

改良法分离培养SD新生乳鼠原代心肌细胞*

目的:建立一种稳定、快速的SD新生乳鼠原代心肌细胞分离培养改良方法。 方法:取SD新生乳鼠心室,0.12%Ⅱ型胶原酶消化,Percoll密度梯度离心结合5-溴脱氧尿嘧啶(5-BrdU)化学抑制法纯化心肌细胞,体外培养于含5%马血清的改良DMEM/F12中,次日更换为普通含10%胎牛血清的高糖DMEM继续培养,并比较此改良方法与传统差速贴壁法的差异。 结果:改良法获得的心肌细胞生长良好,接种24 h 后几乎全部贴壁生长,细胞呈三角形、梭形或不规则形,个别细胞出现自主搏动,频率为10～30 beats/min不等。48 h后心肌细胞变长伸出伪足,部分细胞呈现同步搏动, 频率接近50～80 beats/min。72 h后心肌细胞成菊花样交织成网,自发搏动趋于同步,频率加快至80～100 beats/min;96 h后细胞聚集成簇,呈岛屿样,同步搏动频率在100～120 beats/min左右,一周内细胞状态良好。改良法纯化原代心肌细胞的得率((1.17±0.15)×10⁶ vs (1.21±0.22)×10⁶,P＞0.05)和存活率与传统差速贴壁法相当(93.3%±1.4% vs 92.2%±0.7%, P＞0.05 ),但是改良方法获得的原代心肌细胞纯度更高 (94.7%±2.1% vs 89.5%±1.3%, P＜0.05),且用时较短((3.1±0.4)h vs (4.3±0.3)h, P＜0.01)。 结论:改良法获得心肌细胞耗时短、纯度高、结构功能保存完整,且实验重复和稳定性好,是一种理想且简单易行的的原代心肌细胞分离培养方法。     

Azure a-Schiff, Alcian Blue, HIO4-Schiff, Naphthol Yellow S—A Sequential Staining Method for Paraffin Sections

Paraffin sections from tissue fixed 4-12 hr in 10% formalin containing 0.5% cetyl pyridinium chloride, and washed 2 hr, were stained as follows: (1) Hydrolyze in 5 N HCl at room temperature for 8.5-9 min, or use standard Feulgen hydrolysis at 60 C. (2) Stain in azure A-Schiff, 0.5% in bisulfite bleach (1 N HCl, 5; 10% Na₂S₂O₅, 5; and distilled water 90—parts by volume) for 10 min. (3) Place in bisulfite bleach 2 changes, 2 min each; wash in water, 1-2 min. (4) Stain in Alcian blue (0.1% in 0.01 2V HCl, pH 2.0) for 10 min. (5) Place in 0.01 N HCl for 2-3 min; wash in water for 1-2 min. (6) Oxidize in 0.5% HIO₄ for 5 min; wash in water, 1-2 min. (7) Stain in Schiff's leucofuchsiu, 10 min. (8) Treat with bisulfite bleach as in step 3; wash in running water, 10 min. (9) Stain in naphthol yellow S (0.01% in 1% acetic acid) for 1-2 min. (10) Place in 1% acetic acid for 2 min, dehydrate in tertiary butanol, clear and cover. Result: DNA is deep blue; acidic mucins are light blue; neutral polysaccharides, red to magenta; and proteins, yellow. Proper timing of the hydrolysis for the Feulgen reaction is the most critical step. Overhydrolysis results in green nuclei (staining by naphthol yellow S) whereas purplish nuclei are the results of insufficient hydrolysis.     

Histological Localization of Microelectrode Placement in Brain by Ferrocyanide and Silver Staining

After recordings had been taken from a microelectrode used for mapping nerve impulses, a current of 100 μa from the positive pole of a direct current generator was run through the electrode for 5 sec while it was still in place. On terminating the experiment, in which the use of several electrodes was possible, 50-75 ml of a 1:1 mixture of 4% potassium ferrocyanide and 4% acetic acid was injected into each common carotid artery, and the brain left in situ for 0.5 hr. It was then removed and the electrode-bearing part fixed 5-6 hr in a 1:1 mixture of 40% formalin and 95% ethyl alcohol at 55 °C. This specimen was washed in running water 5-10 min, the electrodes removed and frozen sections of 40-80 μ cut and placed in 95% alcohol. Sections were stained 5-10 min at 25-30°C in 10% silver nitrate solution in 75-80% alcohol acidified by 3-4 drops of glacial acetic acid per 50 ml, washed 4-5 sec in each of 2 baths of 95% alcohol, and reduced while being agitated constantly in a 2% solution of pyrogallol and 6-7% formalin in 75-80% alcohol. Washing in 95% alcohol, clearing in clove oil or methyl salicylate followed by xylene and mounting in synthetic resin or balsam completed the process. Sites of electrolysis at the tips of electrodes (under magnification) were blue before silver staining and black after staining. Axons stained brown to black on a yellow background.     

Effect of bacterial suspensions on vascular occlusion in stems of cut rose flowers

A suspension of Pseudomans aeruginosa at 5 × 10⁹ cfu/ml was either left untreated, pasteurized (15 min, 70°C) or autoclaved (15 min, 121°C). Stems of cut rose flowers ( Rosa hybrida L. cv. Sonia) placed in these solutions for 0·5–4·0 h showed decreased water uptake and a reduction of hydraulic conductance of the basal 5·0 cm stem segment. No difference was found between the treatments. When the pasteurized or autoclaved solutions were left at 4°C for 7 days, bacterial cells had autolyzed, and stems placed in these suspensions showed lower water uptake and hydraulic conductance than stems in freshly prepared solutions. The results show that living and non-living bacteria have the same effect on vascular occlusion, and indicate that hydraulic conductance was more reduced when the average size of the particles was smaller than that of bacterial cells. Vascular blockage occurred within 30 min after the start of treatment, apparently due to a physical effect rather than a physiological response of the stem tissue.     

Staining Germinating Pollen and Pollen Tubes

Germinating pollen on stigmas and pollen tubes in styles of Antirrhinum, Brassica, Oenothera, Raphanus, Rosa, solatium and Tagetes spp. were prepared for examination as follows: The styles were fixed in ethyl alcohol-acetic acid 3:1 for 1 hr, and hydrolyzed at 60°C for 5 to 60 min (depending on the species) in 45% acetic acid. The stigma with its attached strand(s) of stigmatoid tissue was then dissected out under a stereoscopic microscope, placed in a few drops of a staining solution made by dissolving 150 mg of safranin O and 20 mg of aniline blue in 25 ml of hot 45% acetic acid. After 5-15 min in this stain, the tissue was placed in a fresh drop of stain on a microscope slide and gently squashed under a cover glass. Because of a gradual precipitation of the aniline blue component, the stain had to be filtered regularly before use. However, a staining solution could be kept at room temperature for several weeks.     

Selective Staining of Neurosecretory Material in Semithin Epoxy Sections by Gomori's Aldehyde Fuchsin

The epoxy resin was removed from semithin (1 μm) sections by immersing them for 30 sec in sodium methoxide (Mayor et al., J. Biophys. Biochem. Cytol., 9: 909-10, 1961) and then processed as follows: (1) left for 1-3 hr at 60 C in a mixture of formalin, 25 ml; glacial acetic acid, 5 ml; CrO₃, 3 gm; and distilled water, 75 ml: (2) oxidized 10 min in a 1:1:6 v/v mixture of 2.5% KMnO₄, 5% H₂SO₄ and distilled water: (3) bleached in 1% oxalic acid, and (4) stained for 15 min in aldehyde fuchsin, 0.125% in 70% alcohol, or in a 1% aqueous solution of toluidine blue. The neurosecretory material is selectively stained.