A Trichrome Stain for Insect Material

Deparaffinized insect sections are brought down to water and overstained in a 0.1% solution of azocarmine G in 1% acetic acid. They are then destained in a saturated solution of orange G until the azocarmine G is removed from the endocuticle and the latter is colored pale yellow. After washing, the sections are transferred to a 5.0 % solution of phosphotungstic acid in water for 3 min. They are then rinsed in distilled water and stained in a 0.1% solution of methyl green in 1% acetic acid until the endocuticle is green. Differentiation is done in 2 changes of 95% alcohol. The sections are then dehydrated either in absolute alcohol or dioxane, cleared in a mixture of “camsal”, eucalyptol, dioxane, and paraldehyde (1:2:2:1), and mounted in Mohr and Wehrle's medium, a mountant of the Euparal type.     

A Trichrome Stain for Insect Material

Deparaffinized insect sections are brought down to water and overstained in a 0.1% solution of azocarmine G in 1% acetic acid. They are then destained in a saturated solution of orange G until the azocarmine G is removed from the endocuticle and the latter is colored pale yellow. After washing, the sections are transferred to a 5.0 % solution of phosphotungstic acid in water for 3 min. They are then rinsed in distilled water and stained in a 0.1% solution of methyl green in 1% acetic acid until the endocuticle is green. Differentiation is done in 2 changes of 95% alcohol. The sections are then dehydrated either in absolute alcohol or dioxane, cleared in a mixture of “camsal”, eucalyptol, dioxane, and paraldehyde (1:2:2:1), and mounted in Mohr and Wehrle's medium, a mountant of the Euparal type.     

Differentiation of Myofibrillae, Reticular and Collagenous Fibrils in Vertebrates

A procedure for the differentiation of the mesenchymal derivatives, myofibrillae, reticular and collagenous fibers is presented. Formol-Zenker fixation (5-12 hours) is followed by the washing, iodinization, dehydration and paraffin embedding steps routine for that fixative with the following modifications. Zirkle's butyl alcohol series is used for dehydration and infiltration with paraffin as well as in the alcohol slide series. Embedding paraffin used is Parawax plus 8-10% bayberry wax. Tissue-exposed surface of paraffin block is soaked in water overnight before cutting serial sections at 3-5μ. Sections are mounted using the dilute albumen method, and the slides, thoroughly dried at 37^oC. overnight, are left at 60^o for 10 minutes to melt the paraffin of the sections. Before staining, the sections are given a preliminary treatment with potassium permanganate and oxalic acid. For reticular staining a 10% silver nitrate bath is succeeded by an ammoniacal silver carbonate solution followed by reduction in 1% neutral formalin, toning in gold chloride and fixing in sodium thiosulphate. Myofibrillae, the sacroplasmic limiting membrane and other sarcous elements are stained by Heidenhain's azocarmine solution, adult tissues at room temperature and fetal tissues at 50 ^oC. Differentiation in phosphotungstic acid is followed by the staining of collagenous fibers. For adult tissue, light green SF (C.C.) is used and for fetal tissue, fast green FCF (C.C). A discussion of the preparation of ammoniacal silver solutions is included. Both stock and used solutions of ammoniacal silver have been in use by the author for over a period of two years.     

Identification of Medieval Human Soft Tissue Remains in an Advanced State of Decomposition

Naturally preserved human soft tissue remains from mediaeval burials (ll-13th century A. D.) were investigated histologically after azocarmine/aniline alcohol (AZAN) or keratin-prekeratin-mucin (KPM) staining. The tissue remnants were in an advanced state of decomposition; they were completely collapsed and had lost their macroscopic characteristics. After rehydration, thin sectioning, and staining, microscopic properties permitted tissue identification, although differential staining of tissue components did not necessarily correspond with the expected results based on fresh tissue. The techniques and results presented in this paper are relevant for both anthropological and forensic purposes.     

Staining Nerve Fibers with Silver in Tissue Fixed with Bouin's Fluid

Nerve fibers, in organs fixed with Bouin's fluid, are usually refractive to the Davenport silver technic. The axons, however, can be successfully stained if the sections, on slides, are given a preliminary treatment with concentrated pyridine (1 hour), then a 24-hour bath of ammoniated alcohol (99 cc. 80% alcohol, 1 cc 28% ammonium hydroxide) and an interval in 40% aqueous silver nitrate (6-8 hours) before being immersed in the acidified alcoholic silver solution of Davenport. Following the silvering, reduction and toning of the axons, according to the procedure of Davenport, the surrounding non-nervous tissue elements can be counterstained with a combination of either azocarmine, light green and orange G, or azocarmine, aniline blue and orange G.     

Quirks of dye nomenclature. 11. Safranine and its relatives

Safranine was one of the earliest coal tar dyes following mauveine. By the end of the 19th century, many alkylated derivatives of safranine had been made. The history, identity, names, manufacture, analysis, toxicity, textile dyeing, and biological staining applications, plus some nonstaining uses of safranine, phenosafranine, methylene violet, amethyst violet, azocarmine, and Magdala red are described here.     

Differentiation of Two Classes of Acidophiles in the Anterior Pituitary of the Female Rabbit and Cat

A differential stain for the anterior pituitary of mammals, based directly on Heidenhain's 'azan' modification of Mallory's connective tissue stain has been devised. Tissue is fixed for 24 hours in a saturated solution of corrosive sublimate in physiological saline (90 parts) and formalin (10 parts) and washed directly in 70% alcohol for 48 hours. Sections are treated on the slide with a 3% solution of potassium bichromate for 12 hours. Two classes of acidophiles are demonstrated: one which stains selectively with azocarmine; and the ordinary acidophile which stains with orange G. The special acidophile has been demonstrated in the female rabbit and cat but has not been found in the mouse or rat.     

Bismuth Hematoxylin Stain for Arginine Residues

Bismuth ions complex with hematoxylin oxidized by sodium iodate to form a dark blue dye that stains structures with high arginine content. In citrate buffer at pH 5.2, staining is confined to cell nuclei and myelin sheaths. Extraction of nucleic acids has little effect on the stain. Blockade of the guanidino groups of arginine completely abolishes staining.     

Intramitochondrial bodies in sheep adrenal zona glomerulosa cells

Summary Relatively large, mostly rounded, very electron dense intramitochondrial bodies in adrenal zona glomerulosa cells of sheep are described and their nature and connection to protein in the mitochondria discussed. The so called azocarmine granules seen in the light microscope may be identical with the intramitochondrial bodies in the zona glomerulosa cells.     

The influence of ouabain on the elimination of injected and orally applied dyes in Drosophila hydei

The sour dyes azocarmine and indigocarmine are excreted through the Malpighian tubules and the midgut after injection into the body cavity of third instar Drosophila hydei larvae. After injection, the other organs are free of dyes. The epithelium of the midgut does not allow orally applied dyes to pass into the haemolymph. Ouabain diminishes significantly the content of dyes in the cavity of the Malpighian tubules and of the midgut. The maximal concentration of azocarmine decreases in the Malpighian tubules to about 65 per cent and in the midgut to about 70 per cent. Indigocarmine decreases in the Malpighian tubules to about 55 per cent. The content of indigocarmine of the midgut does not change significantly after ouabain injections. As ouabain inhibits active ion transport, the decrease of the concentration of dyes is seen as proof of the coupling of active ion transport processes and of excretion of the dyes. Moreover, this decrease points to an ouabain-sensitive transport mechanism, which is localized in the epithelia of the Malpighian tubules and midgut.     

Evidence on the cellular source of luteotrophin derived from a study of rat pituitary autografts

Summary Pituitary autografts placed under the renal capsule of adult female rats in estrus were found to produce luteotrophin. Indirect evidence indicates that autografts in male and female rats which were operated on at puberty probably produce this hormone also. Studies on both the adult and pubertal animals indicate that pituitary autografts produce the other anterior lobe hormones either at a very low level or not at all.The predominant chromophilic cell type in grafts known to be producing luteotrophin is an elongated acidophile staining selectively with orange G when the azan stain is used. Two types of acidophiles were found in the intact rat pituitary, one staining with azocarmine and the other with orange G. The latter has the same morphology as the predominant cell type in active autografts and is considered to be the source of luteotrophin in the rat.This study was supported by research grant R. G. 4723 from the U.S. Public Health Service.     

Pseudoisocyanin Staining of Insulin and Specificity of Empirical Islet Cell Stains

Two closely related pseudoisocyanins, N,N'-diethyl-6,6'-dichlorpseudoisocyanin chloride and N, N'-diethylpseudoisocyanin chloride, were tested for their metachromatic staining behavior with oxidized insulin. N,N'-diethyl-6,6-dichlorpseudoisocyanin chloride gave nonspecific metachromasia with collagen, mucus, and mast cells of adult tissues; almost all tissues of rat embryos exhibited nonspecific staining. Nonspecific reactions were rarely observed in adult or fetal tissues with the extremely labile metachromasia of N, N'-diethylpseudoiso-cyanin chloride. When oxidation time and temperatures are carefully controlled, this reagent apears to be highly specific for insulin-containing cells and can be used as a selective stain for beta cells. Paraffin sections of formalin fixed material were oxidized 45 sec at 28-29 C in freshly prepared acidified permanganic (2.5% KMnO₄, 1; 5% H₂SO₄, 1; distilled water, 7—parts by volume), decolorized 30 sec in 5% oxalic acid, and washed 5 min in running tap water. After rinsing in 2 changes of distilled water, sections were stained 20 min in a 36 mg/100 ml aqueous solution of N, N'-diethylpseudoisocyanin chloride. Sections were then washed in running tap water until the albumen adhesive was decolorized, and mounted in Karo syrup diluted with an equal amount of distilled water. The insulin-containing cells are stained light to dark purple; all other tissue components, various shades of red. N, N'-diethylpseudoisocyanin chloride was used as a reference for evaluating the specificity of 5 commonly used empirical methods for demonstrating alpha and beta cells in pancreatic islets. Cells exhibiting pseudo isocyanin metachromasia were stained selectively by aldehyde-fuchsin, Heidenhain's azan, and chrome-hematoxylin. Aldehyde-Iuchsin was the only empirical stain tested which gave results comparable to pseudoisocyanin for clarity and definition of beta cells. After oxidation in acidified permanganate, azocarmine and phosphotungstic acid-hematoxylin differentially stained alpha cells; cells demonstrated by these two methods did not exhibit pseudoisocyanin metachromasia. This histochemical procedure can precede empirical methods which require preliminary oxidation in acidified permanganate or it can follow empirical methods which do not extract the insulin nor alter its intramolecular disulfide bonds.     

Hydrogenase activity of Chlorella vulgaris cells

Cell suspensions of Chlorella vulgaris were found to possess the hydrogenase activity as was confirmed by their ability to absorb H2 in the presence of benzyl viologen, azocarmine and other hydrogen acceptors as well as to produce H2 from reduced methyl viologen. Incubation of the cells in the dark under anaerobic conditions in the atmosphere of H2, N2 or Ar stimulated the activity of hydrogenase and induced its de novo synthesis. Treatment of the cells adapted to anaerobiosis with dry ice or liquid nitrogen considerably increased their hydrogenase activity. The enzyme of the adapted cells was more resistant to the inactivation by O2 and temperature.     

血管升压素对大鼠背根神经节神经元膜的作用

为研究血管升压素(arginine vasopressin,AVP)对大鼠背根神经节(dorsal root ganglion,DRG)神经元的作用及其机制,用细胞内微电极记录技术记录离体灌流DRG神经元的膜电位。结果如下:(1)在受检的120个细胞中,大多数(81.67％)在滴加AVP后产生明显的超极化反应。(2)滴加AVP(10μmol/L)后膜电导增加约19.34％(P<0.05)。(3)灌流平衡液巾的NaCl以氯化胆碱(CH-Cl)置代和用Cd2+阻断Ca2+通道后,AVP引起超极化反应的幅值均无明显变化(P>0.05),而加入K+通道阻断剂四乙铵(TEA)后,AVP引起的超极化反应幅值明显减小(P<0.05)。(4)AVP引起的超极化反应可被AVP V.受体拈抗剂阻断。结果捉示,AVP可使DRG大多数神经元膜产生超极化,DRG神经元膜上存在AVP V,受体,且AVP引起的超极化反应是通过神经元膜上AVP V.受体介导的K+外流所致.AVP可能参与了初级感觉信息传入的调制。     

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.     

Unassisted refolding of urea-denatured arginine kinase from shrimp Feneropenaeus chinensis: evidence for two equilibrium intermediates in the refolding pathway

The refolding process and the equilibrium intermediates of urea-denatured arginine kinase (AK) were investigated by 1-anilino-8-naphthalenesulfonate (ANS) intrinsic fluorescence, far-UV circular dichroism (CD), size-exclusion chromatography (SEC), and enzymatic activity. In dilute denaturant, two equilibrium refolding intermediates (I and N') were discovered, and a refolding scheme of urea-denatured AK was proposed. During the refolding of urea-denatured AK, the fluorescence intensity increased remarkably, accompanied by a significant blue shift of the emission maximum and a pronounced increase in molar ellipticity of CD at 222 nm. The first folding intermediate (I) was inactive in urea solution ranging between 2.4 and 3.0 M. The second (N') existed between a 0.4- and 0.8-M urea solution, with slightly increased activity. Neither the blue shift emission maximum nor the molar ellipticity of CD at 222 nm showed significant changes in these two regions. The two intermediates were characterized by monitoring the ANS binding ability in various residual urea solutions, and two peaks of the emission intensity were observed in urea solutions of 0.6 and 2.8 M, respectively. The SEC results indicated that a distribution coefficient (K(D)) platform existed in urea solutions ranging between 2.4 and 3.0 M urea, suggesting that there was a similarly apparent protein profile and size in the urea solution region. The refolding kinetics showed that the urea-denatured AK was in two-phase refolding. Proline isomerization occurred in the unfolding process of AK, which blocked the slow phase of refolding. These results suggested that the refolding process of urea-denatured AK contained at the least two equilibrium refolding intermediates.     

A Simple and Highly Reproducible Staining Method for Fungi and Other Polysaccharide-Rich Microorganisms in Animal Tissues

A newly devised, simple and highly reproducible method for fungal staining is reported. Grocott's method, in which methenamine-silver nitrate solution is employed, has been widely used for the staining of fungi in tissue sections, but it frequently produces heavy background staining because of sudden and progressive reaction in the methenamine-silver nitrate solution. We therefore replace the latter solution with an ammoniacal silver nitrate solution. This new method yields more consistent results in fungal staining without background staining, since the reaction time in die ammoniacal silver nitrate solution is prolonged. The present method is considered superior to Grocott's method with regard to its simplicity and reproducibility.     

Suppression of Costaining of Nonnervous Tissue in Protargol Technics

If, in the procedure of staining nerve fibers in mounted paraffin sections with Protargol according to Bodian, the reduction after toning with gold chloride is executed in a solution of 3-6 drops of aniline oil in 100 ml of 50% alcohol instead of in the prescribed oxalic acid solution, the selectivity of the staining of peripheral nerves is increased. This is effected by a reduction in the intensity of the staining of nonnervous tissue elements. However, at the same time the staining of nonnervous tissue is richer in details and consequently more satisfactory from a histological point of view than it is according to the original method of Bodian or the modification of this method by Ziesmer (1951).     

A simple and highly reproducible staining method for fungi and other polysaccharide-rich microorganisms in animal tissues

A newly devised, simple and highly reproducible method for fungal staining is reported. Grocott's method, in which methenamine-silver nitrate solution is employed, has been widely used for the staining of fungi in tissue sections, but it frequently produces heavy background staining because of sudden and progressive reaction in the methenamine-silver nitrate solution. We therefore replace the latter solution with an ammoniacal silver nitrate solution. This new method yields more consistent results in fungal staining without background staining, since the reaction time in the ammoniacal silver nitrate solution is prolonged. The present method is considered superior to Grocott's method with regard to its simplicity and reproducibility.     

Naphthalene Black Staining of Granules of Eosinophilic Granulocytes: Proposed Mechanism of Action Using Chemical Blockade and Computer Graphics

Histochemical staining of the granules of eosinophilic granulocytes and subsequent blockade of the reaction by alkaline benzil was strongly suggestive that in its purified form, the diazo dye naphthalene black reacts with tissue sites containing high concentrations of arginine residues. Computer graphics modelling indicated that the sulfonate group of the dye reacts electrostatically with the guanidino functional group of arginine. This acid-base type reaction likely has a stoichiometric ratio of 2:1 in favor of the amino acid.