Protective Paraffin Infiltration of Soft Tissues in Insects to Facilitate Softening of Hard Exoskeletons

This technique can produce serial sections as thin as 5 μ from hard chitin-covered materials of insects or other arthropods. Procedures: Fix with alcoholic Bouin's fluid for 3 hr. Henceforth subject material to partial vacuum in each step to ensure a final proper embedding. Wash with 80% ethanol 2 or 3 times for 2 hr or until the picric acid is largely removed. Dehydrate to 90% ethanol and give 2 changes of n-butanol 2 hr each, and one of a 1:1 n-butanol-paraffin mixture in 56-57° oven for 12 hr. Finally, use 2 baths of pure paraffin, 3 hr each, to complete the infiltration. After the last bath, withdraw the specimen from the paraffin, and remove the superficial paraffin, first mechanically and then with a xylene bath for 4 min. Rinse first with n-butanol, and afterwards with absolute ethanol, 2 min each. The compound eyes are protected with a paraffin covering, the specimen is hydrated with a 1% aqueous solution of detergent for 1 hr and then washed with running tap water. The material is treated with a concentrated sulfuric-nitric mixture (H₂SO₄:HNO₃) for 4 hr to eliminate the exoskeleton. After this treatment, the specimen is washed with running tap water for 12 hr, dehydrated with acetone and then bathed in a 2% solution of celloidin in ethyl acetate to form a protective artificial cuticle. This coating is hardened with 2 quick baths of chloroform, the specimen reembedded in paraffin, and the block cast for sectioning.     

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.     

A Durable Nissl Stain for Frozen and Paraffin Sections

Frozen sections, 25-50 /j. thick, of formalin-fixed nervous tissues are mounted following the Albrecht gelatin technic. Paraffin sections, 15 p., are deparaffinized and transferred to absolute ethanol. The slides are then coated with celloidin. Both frozen and paraffin sections subsequently follow the same steps: absolute ethanol-chloroform (equal parts) for at least 20 min, 95% ethanol, 70% ethanol (1-3 min), then rinsed in distilled water. Sections are stained in Cresylechtviolett (Chroma) 0.5% aqueous solution containing 4 drops of glacial acetic acid per 100 ml, rinsed in distilled water, agitated in 70% ethanol until excess stain leaves the slide, and rinsed in 95% ethanol. Sections are then dehydrated in absolute ethanol, followed by butanol, cleared in xylene, and enclosed in permount.     

Adaptation of the Millon, Sudan Black B, and Periodic Acid-Schiff Technics for Block Staining of Insect Tissues

Spermatophores and reproductive systems of the beetle, Lytta nuttalli Say, fixed in Bouin's aqueous picroformol or buffered 10% neutral formol were stained in toto by the Millon, Sudan black B and periodic acid-Schiff reactions as follows. Millon: after excess fixative is removed in 70% ethanol, specimens are brought to water, stained in Millon's reagent at 60 C for 1 hr, rinsed in 2% aqueous nitric acid at 40-50 C, dehydrated rapidly, cleared, embedded and sectioned as usual. Sudan black B: specimens are taken to absolute ethanol, stained in a saturated solution of Sudan black B in absolute ethanol at room temperature for 24-48 hr, rinsed and cleared in xylene, embedded and sectioned. PAS: specimens are brought to water, oxidized in 0.5 aqueous HIO₄ at 37 C for 30 min, washed in 2 changes of water, stained in Schiif reagent at room temperature for 1 hr, rinsed in 3 changes of 0.5% aqueous potassium metabisulfite, washed in running water for 10-15 min, dehydrated, cleared, embedded and sectioned. All 3 methods produced their characteristic staining in specimens up to 3 mm thick     

Techniques for Preparing and Staining Phytophthora Oospores in Soybean Rootlets

Nylon mesh tissue carriers were constructed to hold soybean rootlets through fixing, dehydrating and embedding. Mesh pieces three centimeters square were doubled and sealed at each end by heat. Tissue samples were placed inside with an identifying piece of aluminum foil and the carrier sealed. Rootlets were fixed in Karpechenko's solution, dehydrated in an alcohol series and infiltrated with paraffin. They were embedded in paraffin after removal from the carrier, and sectioned on a microtome. Sections were mounted on glass slides and deparaffinized. A new stain was developed to differentiate oospores of Phytophthora megasperma var. sojae formed in these rootlets. The stain was prepared by dissolving 100 mg bromphenol blue in 50 ml of 95% ethanol and adding 3 g silver nitrate. Procedure: 5 sec in 95% ethanol, 30 min in silver stain, tap water rinse, 5 sec in 95% ethanol, 1 sec in saturated methylene blue in ethanol, immediate rinse in tap water, dehydration in absolute ethanol, rinse in tertiary butanol and xylene and mount. Previous clearing of the tissue was not required, and no air bubbles accumulated within the mesh carrier. This low cost, permeable carrier preserved the minute tissue specimens throughout processing, and the simple, progressive stain clearly differentiated oospores from surrounding tissue.     

Camwood (Baphia nitida) Extract as a Histological Stain for Interglobular Dentine, Striated Muscle, and Counterstaining

The shavings of the dried heartwood of the tree Baphia nitida are ground to a fine powder, and 6 gm of the powder are extracted in 100 ml absolute ethanol at 27-30 for 6-24 hr. The extract is filtered with Whatman No. 1 paper and stored in a screw-capped bottle. For staining the interglobular dentine of nondecalcified sections of formlin-fixed teeth, sawed cross sections 20-30 μ thick were dehydrated in ethanol and stained in the undiluted extract for 6-12 hr at room temperature. The interglobular dentine was stained a bright golden brown on a pale brown background. For staining striated muscle, the extract was diluted 1:1 with distilled water and filtered. After mordanting formalin-fixed paraffin sections with 0.25% KMnO₄ for 5 min, and bleaching with 5% oxalic acid for 10 min, they were washed in water and stained for 2-24 hr at room temperature. The striations were stained light to deep golden brown. For use as a counterstain, a 1:6 dilution of the original extract was required. When applied after haematoxylin for 15-30 min, it stained tissue components in varying shades of golden brown with distribution comparable to that produced by 1% eosin.     

Novel Fixation of Plant Tissue, Staining through Paraffin with Alcian Blue and Hematoxylin, and Improved Slide Preparation

Onion (Allium cepa) root tips were fixed in a proprietary solution without aldehyde, toxic metals or acetic acid. Fixed specimens were embedded in paraffin, sectioned on a rotary microtome and mounted on detergent-washed slides without adhesive. Slides with ribbon segments affixed were immersed in 0.2% aqueous alcian blue 8GX in screw-capped Coplin jars in a water bath at 50 C for 1 hr. Excess alcian blue was rinsed off under cold running tap water and the slides were immersed in quick-mixed hematoxylin at room temperature for 15 min. Stained slides were deparaffinized, rinsed with isopropanol, air dried, and coverslips were affixed with resin. Thus, the traditional paraffin microtechnique has been modified at all steps from fixation to finishing slides with coverslips.     

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.     

Hydroxyethyl Methacrylate Combined with Polyethylene Glycol 400 and Water; an Embedding Medium for Routine 1-2 Micron Sectioning

Pieces of tissue, with the largest dimension not exceeding 7 mm, are fixed and dehydrated by the procedures of choice. Two stock solutions: A, for infiltration; and B, the accelerator, are used in embedding. Formulas: A, 80 ml of glycol methacrylate (2-hydroxyethyl methacrylate—Rohm and Haas Co., Philadelphia, Pa.) is mixed well with 12 ml of polyethylene glycol (Carbowax) 400 and 8 ml of water; then 0.27 gm of benzoyl peroxide added, heated to dissolve the peroxide, and allowed to cool to room temperature. B, polyethylene 200 or 400, 15 parts, and N,N-dimethylaniline, 1 part, mixed thoroughly. Tissues are first infiltrated completely with solution A, then cast in a mixture consisting of 42 parts of A mixed with 1 part of B. Polymerization occurs in 45 min to 3 hr, depending on the temperature. In a water bath at 20 C, the time required was found to be about 3 hr; at 25 C, 1.5 hr; and at 30 C, 45 min. The plastic block can be trimmed easily, and sections 1-2 μ thick readily cut. Sections can be attached to slides by water flotation, without adhesive, and should be dried at room temperature. Staining with aqueous solutions of basic and acid dyes, without removing the embedding matrix, is sharp and brilliant. When staining of the matrix by basic dyes occurs, this background stain can be completely removed by differentiating in either 2-butoxyethanol, pure ethanol, or a mixture of the two. A number of histochemical reagents have been found compatible with this embedding procedure.     

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.     

Brazilin-Toluidine Blue O and Hematoxylin-Darrow Red Methods for Brain and Spinal Cord

Tissue fixed in 10% formalin, formalin-95% ethanol 1:s CaCO₂ or phosphate buffer neutralized formalin, or methanol-chloroform 2:1, was dehydrated and embedded in paraffin or double-embedded by infiltration in 1% celloidin followed by a chloroform-paraffin sequence. Sections were attached to slides with either albumen or gelatine adhesive and processed throughout at room temperature of 24-26 C. For either method, mordanting 30-60 min in 1% iron alum was followed by a 10 min wash in 4 changes of distilled water. For brazilin-toluidne blue O, myelin was stained for 20-60 min, depending upon section thickness, in a self-differentiating solution consisting of: 0.15% Li₂CO₃ 75 ml; 6% brazilin in 95% ethanol, 25 ml; and NaIO₃ 75 mg. After a thorough washing, Nissl material was stained for 3-8 min in a solution consisting of: 0.1 M acetic acid, 90 ml; 0.1 M sodium acetate, 10 ml; and 1% toluidine blue 0, 2.5 ml. For hematoxylin-Darrow red, myelin was stained for 2-6 hr in a self-differentiating solution consisting of: 0.15% Li₂,CO₃ 95 ml; 10% hematoxylin in 95% ethanol, 5 ml; and NaIO₃ 25 mg. After a thorough washing, Nissl material was stained for 20 min or less in a solution consisting of: 0.1 M acetic acid, 90 ml; 0.1 M sodium acetate, 10 ml; Darrow red, 25 mg. This mixture was first boiled, cooled to room temperature and filtered. In both methods, washing, dehydration, clearing, and mounting completed the process. In the brazilin-toluidine blue technic, myelin sheaths were stained reddish purple; neuronal nuclei light blue with dark granules of chromatin; nucleoli dark blue; and cytoplasm blue with dark blue Nissl granules. In the hematoxylin-Darrow red procedure, myelin sheaths were blue-black; nuclei light red with dark granules of chromatin; nucleoli almost black; and cytoplasm red with bright red Nissl granules.     

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.     

Chromosome Spreading Induced by Vegetable Oils

Seeds soaked in the oil extracted from castor beans (Ricinus communis) for 2 hr were germinated in petri dishes on moist filter papers. Root tips were fixed in acetic alcohol (1:3) at 10-14°C, for 24 hr, washed successively with 70% alcohol (15 min) and water (10 min), hydrolysed in 1 N HCl at 60°C for 15 min and stained in leucobasic fuchsin for 30 min. The stained tip was squashed under a cover glass in a drop of acetocarmine and sealed with paraffin wax. The slides were made permanent by separating the cover glass in a mixture of acetic acid and n-butyl alcohol (1:1), passing through 2 changes of n-butyl alcohol and mounting in balsam. Such a method leads to contraction and spreading of chromosomes, without affecting either the clarity of the constriction regions or the anaphase separation of chromosomes.     

Counterstaining Golgi-Cox Impregnations with Luxol Fast Blue as a Myelin Stain

Immerse pieces of brain tissue 4 wk in solutions A and B, mixed just before use: A. K₂Cr₂O₇, 1 gm; HgCl₂, 1 gm; boiling distilled water, 85 ml. Boil A for 15 min, cool to 2 C and add: B. K₂CrO₄, 0.8 gm; Na₂WO₄, 0.5 gm; distilled water, 20 ml. Rinse in water and immerse 24 hr in LiOH, 0.5 gm; KNO₃, 15 gm; distilled water, 100 ml. Wash 24 hr in several changes of 0.2% acetic acid and then for 2 hr in tap water. Dehydrate and embed in celloidin. Process a 60 μ section through 70 and 95% ethanol, a 3:1 mixture of absolute ethanol and chloroform, and toluene. Immerse it for 5 min in a solution containing methyl benzoate, 25 ml; benzyl alcohol, 100 ml; chloroform, 75 ml. Orient the section on a chemically clean slide and let air-dry 5-10 min. Process through toluene, 3:1 ethanol-chloroform and 95% ethanol. Place the section for 5-60 min at 60 C in a solution made up of: Luxol fast blue G (Matheson, Coleman and Bell), 1 gm; 95% ethanol, 1000 ml; 10% acetic acid, 5 ml. Hydrate to water and immerse in 0.05% Li₂CO₃ for 3-4 min. Differentiate in 70% ethanol and place in water. Immerse for 5-15 min in a mixture of two solutions: A. cresylechtviolet (Otto C. Watzka, Montreal), 2 gm; 1 M acetic acid, 185 ml; B. 1 M sodium acetate, 15 ml; distilled water, 400 ml; absolute ethanol, 200 ml. Dehydrate to 3:1 ethanol-chloroform. Clear in toluene and apply a coverslip. The technique produces fast Golgi-Cox impregnated neurons against a background of counterstained myelinated fibers. Patterns of the myelinated fibers can be used to localize impregnated neurons.     

A new fixative solution to precede the reduced silver impregnation of arthropod central nervous systems.

Arthropod central nervous tissue is fixed for 1 hr at 20 C in 8% pure formic acid in 1:1 n-butanol/n-propanol prepared immediately before use (FBP), then washed for 15-30 min in 90% ethanol, and embedded in paraffin wax. Impregnation is by modified Ungewitter techniques in which the silver bath is preceded by mercury/cobalt mordanting, or by modified Holmes' methods following similar mordanting procedures. The methods yield high resolution of axons with minimal background staining, while the staining of neuronal somata is suppressed. They succeed with brains of crustacea and Odonata and other difficult materials. Tissues fixed in FBP are hard and require care in sectioning.     

Immunofluorescence Microscopy of Cyanurated Tissues

Test tissues consisted of: (1) popliteal lymph nodes of rabbits, removed 6 hr after injection of hind footpads with 0.2 ml of 125 mg/ml solution of 5× crystallized chicken ovalbumin, and (2) lungs from guinea pigs, passively sensitized with rabbit antiovalbumin serum, then anaphylactically shocked by intracardial injection of a 1% chicken ovalbumin solution. Similar control tissues from normal rabbits, and lungs of passively sensitized guinea pigs, but shocked with histamine instead of ovalbumin, were included. Pieces of fresh tissue not exceeding 2 mm³ were fixed as follows: (1) Cyanuration—lymph nodes, 1 hr; lung, 0.5 hr; both at 23-27 C—in anhydrous methanol containing 0.5% w/v cyanuric chloride and 1% v/v N, N-diethylaminoethanol. (2) Control fixatives—all specimens 18-24 hr at 4—6 C—absolute methanol; 95% ethanol; neutral buffered 10% formalin; and an FAA mixture (formalin, conc., 6; glacial acetic acid, 2; 30% ethanol, 92). Freeze-dried material was either left unfixed (a control) or fixed in xylene or toluene containing 0.5% w/'v cyanuric chloride and 1% v/v N, N-diisopropylaminoethanol; time and temperature as for fresh tissues. All tissues were routinely dehydrated, cleared, and vacuum embedded in an ester wax, diethylene glycol distearate, or in paraffin at 52 C. Sections 2-4 μ thick were attached to gelatin-coated slides, the wax removed in petroleum ether, and stained 20 min at 23-27 C in a 0.10% solution of fluorescein isothiocyanate-conjugated rabbit antiovalbumin globulin, washed in phosphate buffered saline 10 min, dehydrated, cleared and covered in a nonfluorescent medium. With ultraviolet illumination, brightly immunofluorescent, anti-genically specific staining was obtained in cyanurated fresh and freeze-dried lymph node and lung tissues. In contrast, specific staining was diminished or absent in comparable tissues reacted in the control fixatives.     

A New Fixative Solution to Precede the Reduced Silver Impregnation of Arthropod Central Nervous Systems

Arthropod central nervous tissue is fixed for 1 hr at 20 C in 8% pure formic acid in 1:1 n-butanol/n-propanol prepared immediately before use (FBP), then washed for 15-30 min in 90% ethanol, and embedded in paraffin wax. Impregnation is by modified Ungewitter techniques in which the silver bath is preceded by mercury/cobalt mordanting, or by modified Holmes' methods following similar mordanting procedures. the methods yield high resolution of axons with minimal background staining, while the staining of neuronal somata is suppressed. They succeed with brains of crustacea and Odonata and other difficult materials. Tissues fixed in FBP are hard and require care in sectioning.     

A Celloidin Infiltration-Frozen Section Sequence for Enhanced Preservation of Phosphatases in Bone

The effect of the following embedding procedures on the acid and alkaline phosphatase content of decalcified mouse tibiae has been studied: embedding in 23% gelatine for 18 hr at 37° C, embedding in paraffin wax in vacuo for 1 hr at 58° C, and impregnation with 4% celloidin in diethyl ether and ethanol at 4° C for 2-3 days. Unsupported tissues were also used to demonstrate these enzymes for comparison with the above procedures. Tibiae were first fixed in 10% neutral formalin at 4° C for 15 hr, decalcified in equal volumes of 2% formic acid and 20% sodium citrate at pH 4.9 for not more than 5 days and then washed in distilled water before carrying out the embedding schedules. The celloidin-impregnated tibiae were placed in 70% ethanol to harden the celloidin and then washed in distilled water for 1-2 hr. These tibiae and those embedded in gelatine were cast in a gelatine block which was then hardened in 10% neutral formalin at 4° C for 2 hr. Sections of these and unsupported tibiae were cut at 15 μ on a freezing microtome. Decalcified tibiae embedded and blocked in paraffin wax were sectioned at 15 μ on a base sledge microtome. The enzymes were demonstrated using the coupling azo dye method given by Pearse (Histochemistry, 1st Ed. 1954). The stable diazotates of 4 benzoyl amino 2-5 diethoxyanilene, 3 nitro toluidine and o-dianisidine were used. Of the embedding procedures paraffin wax embedding produced the greatest loss of both enzymes. Gelatine embedding and infiltration with celloidin were equally good for the demonstration of acid phosphatase but for alkaline phosphatase the celloidin method was superior. The gelatine embedded material did not produce consistently good results. Celloidin-impregnated tibiae could be stored without marked deterioration of the enzyme content for longer than gelatine-embedded tibiae.     

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.     

Improved Procedures in Fungal Cytology Utilizing Giemsa

To study nuclear events in fructifications of the Basidiomycetes, material was fixed 24 hr in a saturated aqueous solution of HgCl₂ containing 1% glacial acetic acid, and embedded in Aquax (G. T. Gurr Ltd.). Following a 4 hr hydrolysis at 20 C in 60% H₃PO₄, sections were stained for 30 min in a mixture of 4 ml Giemsa R66 (G T. Gurr Ltd.) and 100 ml phosphate buffer at pH 6.5. Differentiation was carried out in sodium cacodylate-HCl buffer at pH 5.8 when required. Preparations were dehydrated in an acetone-xylene series prior to mounting in Euparal. The use of paraffin wax as the embedding medium and HCl as the hydrolysing agent yielded preparations of an inferior quality.