Injection of Lymphatics: With Colored Cedar Oil; With Plastic

(1) The oil mass consists of: cedar oil, 1; color in oil (a paint pigment, e.g., Prussian blue), 1; and toluene, 2, parts by volume. To use, add 1 ml of diethyl ether to each 10 ml of mass, mix thoroughly and inject into the fresh organ with a very fine glass or metallic needle. Heat the organ in water at 50-60° C before starting the injection, massage gently after injection, then fix. For macroscopic studies, fix 5 days in 5% formalin, and dissect. For microscopic studies, fix at least 5 days in: formalin, 10 ml; Al₂(SO₄)₃, 2 gm; ZnSO₄, 2 gm; acetic acid, 4 ml; and distilled water, 90 ml. Dehydrate with dioxane, embed in paraffin and section at 10-20 μ. Stain with hematoxylin-eosin or with one of the following modifications of Van Gieson's formula: 1. 1% acid fuchsin, 10; picric acid (sat. aq.), 50; and 5% ZnSO₄, 40 volumes. 2. 1% acid fuchsin, 20; picric acid (sat. aq.), 80; and 5% CoSO₄, 40 volumes.

(2) The plastic mass consists of a 5-10% solution of Rhodopas (a vinyl copolymer) in acetone. Injection is made as with the oil mass except that a plastic squeeze-bottle and glass needle is preferable to a syringe. Indirect injection is used for both procedures, i.e., into the organ substance; not into a cannulated lymphatic vessel. After the plastic has hardened (24 hr), the unfixed tissue is subjected to corrosion by 5-10% NaOH in water.     

Fuchsin staining with naoh clearing for lignified elements of whole plants or plants organs

Three methods that are adapted to the various consistencies of plants are as follows: 1. Samples are placed for 10-14 hr at 60° C in a 1% aqueous solution of basic fuchsin, to which 10 gm of solid NaOH per 100 ml are added. 2. Samples when taken out of 95% alcohol are placed in a 1% solution of basic fuchsin in 95% alcohol for 24 hr; after washing in water, they are placed in a 15% solution of NaOH at 60° C until cleared. 3. Samples are placed in a 15% aqueous solution of NaOH at 60° C until cleared, then for 24 hr at 60° C in 15% NaOH containing basic fuchsin. After being stained and cleared by one of these three methods, the samples are rinsed in water, dehydrated and then passed into a mixture of absolute alcohol and concentrated HC1 (3:1) for 1-15 min, rinsed in absolute alcohol, cleared in xylene and mounted in Canada balsam. The lignified tissues appear red; the others, transparent.     

Differentiated Staining of Osmium Tetroxide-Fixed, Vestopal-w-Embedded Tissue in thin Sections

Tissues were fixed at 20° C for 1 hr in 1% OsO₄, buffered at pH 7.4 with veronal-acetate (Palade's fixative), soaked 5 min in the same buffer without OsO₄, then dehydrated in buffer-acetone mixtures of 30, 50, 75 and 90% acetone content, and finally in anhydrous acetone. Infiltration was accomplished through Vestopal-W-acetone mixtures of 1:3, 1:1, 3:1 to undiluted Vestopal. After polymerisation at 60° C for 24 hr, 1-2 μ sections were cut, dried on slides without adhesive, and stained by any of the following methods. (1) Mayer's acid hemalum: Flood the slides with the staining solution and allow to stand at 20°C for 2-3 hr while the water of the solution evaporates; wash in distilled water, 2 min; differentiate in 1% HCl; rinse 1-2 sec in 10% NH,OH. (2) Iron-trioxyhematein (of Hansen): Apply the staining solution as in method 1; wash 3-5 min in 5% acetic acid; restain for 1-12 hr by flooding with a mixture consisting of staining solution, 2 parts, and 1 part of a 1:1 mixture of 2% acetic acid and 2% H₂SO₄ (observe under microscope for staining intensity); wash 2 min in distilled water and 1 hr in tap water. (3) Iron-hematoxylin (Heidenhain): Mordant 6 hr in 2.5% iron-alum solution; wash 1 min in distilled water; stain in 1% or 0.5% ripened hematoxylin for 3-12 br; differentiate 8 min in 2.5%, and 15 min in 1% iron-alum solution; wash 1 hr in tap water. (4) Aceto-carmine (Schneider): Stain 12-24 hr; wash 0.5-1.0 min in distilled water. (5) Picrofuchsin: Stain 24-48 hr in 1% acid fuchsin dissolved in saturated aqueous picric acid; differentiate for only 1-2 sec in 96% ethanol. (6) Modified Giemsa: Mix 640 ml of a solution of 9.08 gm KH₂PO₄ in 1000 ml of distilled water and 360 ml of a solution of 11.88 gm Na₂HPO₄-2H₂O in 1000 ml of distilled water. Soak sections in this buffer, 12 hr. Dissolve 1.0 gm of azur I in 125 ml of boiling distilled water; add 0.5 gm of methylene blue; filter and add hot distilled water until a volume of 250 ml is reached (solution “AM”). Dissolve 1.5 gm of eosin, yellowish, in 250 ml of hot distilled water; filter (solution “E”). Mix 1.5 ml of “AM” in 100 ml of buffer with 3 ml of “E” in 100 ml of buffer. Stain 12-24 hr. Differentiate 3 sec in 25 ml methyl benzoate in 75 ml dioxane; 3 sec in 35 ml methyl benzoate in 65 ml acetone; 3 sec in 30 ml acetone in 70 ml methyl benzoate; and 3 sec in 5 ml acetone in 95 ml methyl benzoate. Dehydrated sections may be covered in a neutral synthetic resin (Caedax was used).     

Staining of Nervous Tissue by Protein-Silver Mixtures

A staining method for nerves in paraffin sections is described in which an egg albumen-silver nitrate mixture is the impregnating solution. Blocks of tissue are fixed in Bouin's fixative, formol, Huber's fixative or formol-acetic-alcohol, and decalcified if necessary in Bensley's decalcifier. Sections are impregnated overnight, in the dark, at 37-56°C in a solution containing 50 ml of filtered, aqueous 0.5% dried egg albumen with 1.8-2.5 ml of 2% silver nitrate and adjusted to pH 8.2-8.3 by the addition of ammonia. The sections are then rinsed in distilled water and the silver reduced in a mixture of hydroquinone, 1 gm; anhydrous sodium sulfite, 10 gm and distilled water, 100 ml. The remainder of the process consists of washing, gold toning, fixing in 5% sodium thiosulfate, washing, dehydrating, clearing and mounting. Casein may be used as an alternative to egg albumen in the impregnating solution (0.5% casein, 50 ml; 2% silver nitrate, 1 ml). The pH value of the solution may be adjusted by a boric acid-borax buffer or ammonium hydrogen tetraborate in the place of ammonia.     

Softening Paraffin-Embedded Plant Tissues

Soaking paraffin-embedded plant specimens 2-3 days at 37°C. in a mixture of glycerol, 10 ml., Dreft, 1 g., and water 90 ml. is an effective means of softening them prior to sectioning. One side of the paraffin block must be pared away to expose the tissue before immersion in the softening solution.     

Embedding Media for 1-2 Micron Sectioning. 2. Hydroxyethyl Methacrylate Combined with 2-Butoxyethanol

A hydroxyethyl methacrylate monomer medium incorporating 2-butoxyethanol requires 2 stock solutions for embedding. Solution A: 80 ml of hydroxyethyl methacrylate (Rohm and Haas Co., Philadelphia, Pa.) is mixed well with 16 ml of 2-butoxyethanol; 0.27 gm of benzoyl peroxide, the catalyst, is added and permitted to dissolve. Heating to 40-50 C may be used to accelerate its solution. Solution B: polyethylene glycol 200 or 400, 15 parts, and N,N-dimethylaniline, 1 part, are mixed thoroughly. Tissues are dehydrated in the customary manner to absolute ethanol or other comparable dehydrant, infiltrated completely with A, then cast in a mixture consisting of 42 parts of A well mixed with 1 part of B. Polymerizaion occurs in 4-7 hr. In a water bath at 20 C the time required was about 7 hr; at 28 C, 4 hr. This medium is based on the author's water-polyethylene glycol-hydroxyethyl methacrylate monomer medium (Stain Techn., 42: 119-23, 1967).     

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.     

Embedding Media for 1-2 Micron Sectioning. 3. Hydroxyethyl Methacrylate-Benzoyl Peroxide Activated with Pyridine

A hydroxyethyl methacrylate (HEMA) monomer medium containing 2-butoxyethanol as the plasticizer requites only one stock solution consisting of: 50 ml of 94 or 96% HEMA containing 200 ppm inhibitor (Rohm and Haas, Philadelphia) is mixed with 12 ml 2-butoxyethanol; 0.25 gm benzoyl peroxide is added and permitted to dissolve at 20-25 C. This mixture is activated by the addition of 0.8-1.0 ml of pyridine. Polymerization of the activated mixture is initated in 15-20 hr at 25 C and in 2-4 hr at 50 C; polymerization of the mixture is complete in 2-3 days and 3-6 hr, respectively. The activated monomer mixture is stable at temperatures below 18 C; hence infiltration of tissues may be extended to 7-10 days by keeping the mixture at 0 to -40 C.     

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.     

Simplified Aldehyde-Fuchsin Staining of Neurosecretory Cells

Gomori's original aldehyde-fuchsin method has been modified by the combination of Halmi's counter stain with Gabe's preparation, consisting of basic fuchsin, 1 gm; boiling water, 200 ml; with HC1, 2 ml and paraldehyde, 2 ml added after cooling and filtering. The solution so made was allowed to ripen 3-4 days at room temperature, and the precipitate which formed was filtered off and dried at 55-60°C. The staining solution consisted of 0.5 gm of the dry precipitate dissolved in 100 ml of 70% alcohol. The staining follows original procedures except that it is very important to bring slides from water to 70% alcohol before placing them in the aldehyde-fuchsin solution and also to remove all excess staining solution by rinsing in 95% alcohol after staining. The staining solution is stable for at least 6 mo.     

A Plastic Embedding Medium for Thin Sectioning in Light Microscopy

Tissue blocks with surface areas up to 2 cm² can be sectioned at 1 or 2 μ after embedding in a medium consisting of: methyl methacrylate, 27 ml; polyethylene glycol distearate MW 1540, 6 gm; dibutyl phthalate, 4 ml; and Plexiglas molding powder A-100, 9 gm (added last). The methacrylate mixture is polymerized at 50° C by benzoyl peroxide, 0.8 gm/ 100 ml of methacrylate. The polymerized matrix is transparent and the blocks can be cut on a rotary microtome with a steel knife. The plastic can be removed from sections with acetone prior to staining. Artifacts caused by embedding and sectioning are negligible     

A Paraffin Method for Refractory Plant Materials

A modification of Zirkle's n-butyl alcohol method for dehydrating refractory plant material and embedding it in paraffin is described. The material is cut into small pieces and killed and fixed in CRAF III. It is dehydrated in Zirkle's n-butyl alcohol series, slightly modified. Infiltration is accomplished by adding chips of paraffin of low melting point (52°C.) to the bottle containing butyl alcohol and the tissues at a gradually increasing series of temperatures. The butyl-alcohol-paraffin mixture is gradually replaced by pure paraffin (melting point 56-58°C). The material is embedded in Fisher Tissuemat (56-58°C). Before microtoming, the block of embedded tissue is trimmed so that part of the specimen is exposed, and it is soaked in water until it cuts easily.     

Staining Residual Lipids in Ultrathin Sections of Tissues Embedded in Polyester Resin

Rat suprarenal glands fixed in Palade's 1% OsO₄, buffered at pH 7.7 with veronal-acetate, to which 0.1% MgCl₂ was added, were embedded in Vestopal-W and sectioned at 0.2-1 µ. The sections were attached to slides by floating on water, without adhesive, and drying at 60-80° C, placed in acetone for 1 min and then treated with the following staining procedure: Place the preparation in a filtered solution of oil red O, 1 gm; 70% alcohol, 50 ml; and acetone, C.P., 50 ml; for 0.5-1 hr. Rinse in absolute ethyl alcohol; drain; counterstain with 0.5% aqueous thionin for 5 min; rinse in distilled water; drain; stain in 0.2% azure B in phosphate buffer at pH 9, for 5 min. Dry and apply a drop of immersion oil directly on the section. The preparations are temporary. Ciaccio-positive lipids, rendered insoluble by OsO, fixation, stained red to ochre.     

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 temperature on the longevity of human fibroblasts in culture

The longevity of parallel cultures of the human diploid fibroblast strain MRC-5 was measured at various incubation temperatures. At 37°C the mean life-span was 57.2 passages, at 34°C it was 58.7 passages and at 40°C it was 29.2 passages. There was greater variation in longevity among cultures grown at 40°C than in the control population and least among those grown at 34°C. The decreased life-span at 40°C was probably due to accelerated ageing, as the transfer of senescent cultures back to 37°C did not lead to their recovery. Cultures grown at 32°C also had reduced life-span compared to the control, but this was probably not the result of ageing, as the transfer of cultures which had almost ceased growth back to 37°C allowed them to reach the normal life-span for this temperature. The results imply that clonal ageing is at least in part due to random events—possibly errors in protein synthesis—which occur more frequently with increasing temperature.     

Staining and Mounting Helminths

The following procedure is recommended: Fix ces-todes and trematodes (while held flat between glass slides) 0.5-2.0 hr. in the following mixture: formalin, 15; acetic acid (gl.), 5; glycerol, 10; 95% ethyl alcohol, 24; distilled H₂O, 46; all proportions by volume. After freeing them from the slides, wash thoroughly in running water and stain immediately thereafter. Stock staining solution: ferric ammonium alum (violet cryst.), 2 g.; distilled H₂O (cold) 100 ml.; after solution, add 2 ml. concentrated H₂SO₄, bring to a boil; add 1 g. coelestin blue B (Nat. Aniline), boil 3-5 min.; cool and add 10 ml. absolute methyl alcohol and 10 ml. glycerol. Dilute 1 vol. with 3 vol. distilled H20 for use. Stain 5-30 min., depending on size of specimens. Wash with 2 changes 0.5 hr. each of distilled H₂O, then 50% isopropyl alcohol 12-16 hr., 50% isopropyl alcohol 2 hr., followed by graded isopropyl alcohol for dehydration. Ether: ethyl alcohol (equal parts), 1 hr., is followed by embedding in celloidin in a sheet just thick enough to cover the specimens. Trim embedded specimens and dehydrate with isopropyl alcohol, 80%, 90% and absolute. Clear in beechwood creosote. Mount in balsam with cover glasses that overlap the edges of the celloidin 1-2 mm. While drying at 37°C, refill edges of mount with fresh balsam as needed. When dry, remove excess balsam and ring the edges with ordinary gloss enamel paint.     

A Ribonuclease-Gallocyanin Stain for Sexing Skin Biopsies

Skin biopsies for sexing can be fixed best in 10-15% aqueous formalin or this solution saturated with HgCl₂. Bouin's fluid and all chromate mixtures should be avoided. Celloidin-paraffin double embedding is recommended but not essential. Sections are brought to water, mercurial residues removed if necessary, and then washed in distilled water. They are incubated at 37°C in a ribo-nuclease solution: approximately 1 mg of ribonuclease powder (Light's) in 100 ml of glass-distilled water; boiled 3-5 sec after dissolving, and kept in a refrigerator (usable about a week). The sections are rinsed and incubated at 37°C overnight in gallocyanin-chromalum (Einarson, 1951) made as follows: Dissolve 5 gm of chromalum in 100 ml of distilled water, add 0.15 gm of gallocyanin, shake thoroughly, heat slowly and boil 5 min; cool, filter, and wash through the filter with distilled water until the filtrate reaches 100 ml. This solution is usable at once and keeps at least a month. Sections should be dipped in acid alcohol to clean (optional), but no attempt made to differentiate them, and washed in tap water. Dehydration, clearing and covering complete the process. The method is nearly as precise as the Feulgen and more convenient and reliable for routine use on miscellaneous material.     

A Universal Stain for the Sex Chromatin Body

For the demonstration of the sex chromatin body in human tissues, fixation in 95% alcohol or modified Davidson's solution (95% alcohol, 30; formalin, 20; glacial acetic acid, 10; distilled water, 30) was best. The staining procedure chosen for most materials is the following: Mounted preparations are coated with celloidin, hydrated, hydrolyzed 20 min in 52V HCl at 20-25°C, rinsed thoroughly in several changes of distilled water and transferred to a buffered thionin solution. This consists of 3 parts: (1) A saturated solution of thionin in 50% alcohol (filtered); (2) Michaelis buffer: sodium acetate (3 H₂O), 9.714 gm; sodium barbiturate, 14.714 gm; CO₂-free distilled water, 500 ml; and (3) 0.1N HCl. To make the staining solution, mix 28.0 ml of the buffer solution with 32.0 ml of 0.1N HCl and bring the total volume to 100.0 ml with the thionin solution. Its pH should be 5.7 × 0.2, and care should be exercised that no acid is carried over from the hydrolyzing solution, since this would progressively lower the pH. The staining time varies from 15 to 60 min, depending on the specimen, but the shortest time consistent with adequate staining gives the clearest preparations. Slides are rinsed in distilled water and 50% alcohol and allowed to remain in 70% alcohol until the heavy clouds of stain cease to appear. Differentiation is completed in 80% and 95% alcohol, followed by dehydration in absolute alcohol, clearing in xylene and applying a cover glass with a synthetic resin (G. T. Gurr's DePeX was used). The sex chromatin is deep blue-violet and sharply contrasted against the lightly colored particulate chromatin of the nucleus. Cytoplasm remains unstained but fibrin and related structures show metachromasia. Chromosomes are well demonstrated if present. The method works on all types of tissues, is simpler and quicker than the Feulgen method, and often yields superior results.     

The Use of Lacto-Propionic Orcein in Rapid Squash Methods for Chromosome Preparations

A solution of 2 gm of natural orcein dissolved in 100 ml of a mixture of equal parts of lactic and propionic acids, and diluted to 45% with water, proved more effective than other stain fixatives for meiotic preparations from fresh pollen mother cells. When used after 5 min fixation in modified Carnoy's fixative (alcohol, acetic acid, chloroform, formalin; 10:2:2:1) and 5 min maceration in 1 N HC1 at 60° C, the same stain proved the most suitable for the rapid preparation of root-tip chromosomes for counting and for studying detailed morphology.     

Avian Microchromosomes; As Shown by Prefixation Treatment with Colchicine, Squashing, and Haematoxylin Staining

Small pieces of bird tissue from developing feathers, embryos, embryonic gonads and adult testes are treated before fixation in a 0.25% solution of colchicine diluted with an equal volume of hypotonic Pannett and Compton solution containing KCI, 0.336 gm; CaCl₂, 0.160 gm; Na₂HP0₄. 12H₂O, 0.172 gm; and NaH₂PO₄. 4H₂O, 0.0172 gm per 1000 ml of double distilled water, for 20-30 min at 37° C. This material is subsequently centrifuged at 1000 rev/min for 1-3 min, fixed with acetic alcohol (1:3) and stained with either Gomori's haematoxylin or by Feulgen's procedure. Preparations are frozen in the freezing chamber of a refrigerator for the separation of the cover slips, then mounted in euparal after dehydration in alcohols. With this technique, unclumped and clear preparations of both macrochromosomes and microchromosomes are obtained regularly.