Demonstration of Elastic Tissue and Iron or Elastic Tissue and Calcium Simultaneously

For the concomitant demonstration of iron and elastic tissue Perls' test solution was used, followed by Verhoeff's stain or Gomori's aldehyde fuchsin. When Perls' and Verhoeff's stain were used in sequence, the iron deposits were greenish blue and the elastic lamellae were black. When Perls' test solution was combined with aldehyde fuchsin the iron deposits were blue and elastic tissue purple. Calcium salts and elastic tissue were demonstrated concomitantly by using von Kossa's method followed by Gomori's aldehyde fuchsin. With such combined staining, the calcium salts appeared brownish black and elastic tissue purple. With these procedures, it was possible to see the exact relationship of calcium and iron deposits to the elastic tissue.     

Demonstration of Elastic Tissue and Iron or Elastic Tissue and Calcium Simultaneously

For the concomitant demonstration of iron and elastic tissue Perls' test solution was used, followed by Verhoeff's stain or Gomori's aldehyde fuchsin. When Perls' and Verhoeff's stain were used in sequence, the iron deposits were greenish blue and the elastic lamellae were black. When Perls' test solution was combined with aldehyde fuchsin the iron deposits were blue and elastic tissue purple. Calcium salts and elastic tissue were demonstrated concomitantly by using von Kossa's method followed by Gomori's aldehyde fuchsin. With such combined staining, the calcium salts appeared brownish black and elastic tissue purple. With these procedures, it was possible to see the exact relationship of calcium and iron deposits to the elastic tissue.     

Growth of Thiobacillus ferrooxidans on Formic Acid

A variety of acidophilic microorganisms were shown to be capable of oxidizing formate. These included Thiobacillus ferrooxidans ATCC 21834, which, however, could not grow on formate in normal batch cultures. However, the organism could be grown on formate when the substrate supply was growth limiting, e.g., in formate-limited chemostat cultures. The cell densities achieved by the use of the latter cultivation method were higher than cell densities reported for growth of T. ferrooxidans on ferrous iron or reduced sulfur compounds. Inhibition of formate oxidation by cell suspensions, but not cell extracts, of formate-grown T. ferrooxidans occurred at formate concentrations above 100 μM. This observation explains the inability of the organism to grow on formate in batch cultures. Cells grown in formate-limited chemostat cultures retained the ability to oxidize ferrous iron at high rates. Ribulose 1,5-bisphosphate carboxylase activities in cell extracts indicated that T. ferrooxidans employs the Calvin cycle for carbon assimilation during growth on formate. Oxidation of formate by cell extracts was NAD(P) independent.     

Iron Gallein Elastic Method—A Substitute for Verhoeff'S Elastic Tissue Stain

A method for staining elastic fibers in formalin fixed, paraffin embedded sections is described. After deparaffinizing and dehydration. sections are stained for 30 minutes in a solution prepared by mixing equal parts of 1% gallein dissolved in ethylene glycol and absolute alcohol (1:4), and 1.16% aqueous ferric chloride in 1% hydrochloric acid. The sections are washed in water and then differentiated in 2% ferric chloride for 2 minutes. After washing in water, the sections am counterstained with a variant of Van Girson's picric acid-acid fuchsin for 1 minute. The results are similar to Verhoeff s elastic stain with elastic fibers staining black. An advantage to this staining procedure is that visually controlled differentiation is not necessary.     

Correlation Effects in the Double Proton Transfer of the Formic Acid Dimer

The role of correlation effects in the potential energy hypersurface for the double proton transfer in the hydrogen bond of the formic acid dimer has been studied at the non-empirical level. The calculations were performed in different large as well as for the first time in complete basis set at the correlation level. The possible reasons of incorrect results of quantum chemical calculations are considered.     

Screening of Non- Saccharomyces cerevisiae Strains for Tolerance to Formic Acid in Bioethanol Fermentation

Formic acid is one of the major inhibitory compounds present in hydrolysates derived from lignocellulosic materials, the presence of which can significantly hamper the efficiency of converting available sugars into bioethanol. This study investigated the potential for screening formic acid tolerance in non-Saccharomyces cerevisiae yeast strains, which could be used for the development of advanced generation bioethanol processes. Spot plate and phenotypic microarray methods were used to screen the formic acid tolerance of 7 non-Saccharomyces cerevisiae yeasts. S. kudriavzeii IFO1802 and S. arboricolus 2.3319 displayed a higher formic acid tolerance when compared to other strains in the study. Strain S. arboricolus 2.3319 was selected for further investigation due to its genetic variability among the Saccharomyces species as related to Saccharomyces cerevisiae and availability of two sibling strains: S. arboricolus 2.3317 and 2.3318 in the lab. The tolerance of S. arboricolus strains (2.3317, 2.3318 and 2.3319) to formic acid was further investigated by lab-scale fermentation analysis, and compared with S. cerevisiae NCYC2592. S. arboricolus 2.3319 demonstrated improved formic acid tolerance and a similar bioethanol synthesis capacity to S. cerevisiae NCYC2592, while S. arboricolus 2.3317 and 2.3318 exhibited an overall inferior performance. Metabolite analysis indicated that S. arboricolus strain 2.3319 accumulated comparatively high concentrations of glycerol and glycogen, which may have contributed to its ability to tolerate high levels of formic acid.     

Quad-Type Stain for the Simultaneous Demonstration of Intracellular and Extracellular Tissue Components

This technic for the simultaneous demonstration of several different tissue components works equally well on invertebrate and vertebrate tissue if they have been treated with nonchromate fixatives Sections 4-7 μ thick are stained 30 min in 1% Alcian blue, then treated with alkaline alcohol for 2 hr. They are stained in Verhoeff's hematoxylin for 4-6 hr, and rinsed in alcohol; stained in woodstain scarlet-acid fuchsin for 3 min, decolorized in 5% phosphotungstic acid for 20 min and finally stained 5-8 min in alcoholic saffron. Collagen and bone are stained yellow; elastin, myelin and nucleic acids, purple to black; muscle, chitin, cytoplasm, fibrinoid and acid secretion, bright red to lavender; ground substances and mucus, blue-green. Fibrous connective tissue, cartilage, bone and glandular epithelia are exceptionally well demonstrated by this method. Slides stained in this manner are well suited for color photomicrography and as demonstrations in the classroom.     

Formic acid triggers the "Acid Crash" of acetone-butanol-ethanol fermentation by Clostridium acetobutylicum

Solvent production by Clostridium acetobutylicum collapses when cells are grown in pH-uncontrolled glucose medium, the so-called "acid crash" phenomenon. It is generally accepted that the fast accumulation of acetic acid and butyric acid triggers the acid crash. We found that addition of 1 mM formic acid into corn mash medium could trigger acid crash, suggesting that formic acid might be related to acid crash. When it was grown in pH-uncontrolled glucose medium or glucose-rich medium, C. acetobutylicum DSM 1731 containing the empty plasmid pIMP1 failed to produce solvents and was found to accumulate 0.5 to 1.24 mM formic acid intracellularly. In contrast, recombinant strain DSM 1731 with formate dehydrogenase activity did not accumulate formic acid intracellularly and could produce solvent as usual. We therefore conclude that the accumulation of formic acid, rather than acetic acid and butyric acid, is responsible for the acid crash of acetone-butanol-ethanol fermentation.     

Improved Recovery of Somatomedin Activity from Plasma by Prolonged Formic Acid Extraction

Recovery of somatomedin activity from plasma fractions was increased approximately 5-fold by prolonged extraction of isolates with formic acid. Extraction for 72 hours enhanced the yields of active peptides in the 6,000, 8,000 and >20,000 dalton range. Yields of smaller peptides were similar following short (2 hrs) and long (72 hrs) extraction periods. Active fractions obtained after prolonged extraction possessed sulfation activity and insulin-receptor affinity comparable to somatomedin isolated during short extraction with formic acid.     

Some Observations on the Demonstration of Calcium Oxalate in Tissue Sections

Crystal deposits in human kidney and thyroid, identified as calcium oxalate by microincineration and Solubility tents, were used to assess the staining of oxahtes by selected methods for calcium. No method that stained the crystals was considered specific for calcium oxalate, but, after removal of possible phosphate and carbonate with 2 M acetic acid, the silver nitrate-rubeanic acid sequence was found to give the best visualisation of the crystals, and could be considered reasonably selective. Deposits in kidneys included a pronounced colloidal matrix composed chiefly of acid mucopolysaccharides. This matrix often showed a lamellar pattern and was well-demonstrated by alcian blue at pH 25 and by dialysed iron after removal of the crystals with 1 N hydrochloric acid. Such a matrix Could only be detected in trace amount in the thyroid deposits.     

Effect of Indoleacetic Acid on the Abscisic Acid Level in Stem Tissue

Excised stem sections from growing plants of Populus tremula L. and Pisum sativum L. including lateral buds were treated with indole-3-acetic acid in a phosphate buffer solution. In control sections the level of the abscisic acid-like inhibitor decreased strongly during 24 h as did the level of the endogenous auxin. Exogenous indoleacetic acid counteracted the decrease in the inhibitor level to a considerable extent. Implications of this auxin effect in relation to apical dominance are discussed.     

Use of Ethylenediaminetetraacetic Acid in the Cytologic Demonstration of Amylophosphorylase

Ethylenediaminetetraacetic acid (EDTA) was found to enhance strikingly the staining reaction of rat livers to the Takeuchi and Kuriaki method for phosphorylase (J. Histochem. Cytochera., 3: 153, 1955). Frozen sections of rat livers were prepared as described previously (S. H. Hori, Stain Techn., 39: 275, 1964), incubated in the medium containing: glucose-1-phosphate, 6 mM; adenosine-5-phosphate, 0.3 mM; EDTA, 20 mM; acetate buffer, pH 5.8, 80 mM, and the stain, developed with an aqueous solution of I₂-KI, 1:2:300. The result obtained with this technique was similar to that with the lead technique of the author, but it showed a more intense reaction in centrolobular areas than in periportal areas.     

A Method for the Selective Removal of Deoxyribonucleic Acid from Tissue Sections

The deoxyrihonucleic acid (DNA) of chromatin undergoar depurinization on mild acid hydrolysis with a picric acid-formaldehyde mixture (Bouin's fluid). The apurinic acid thus formed is degraded by condensation with aniline and is lost from tissue sections, but ribonucleic acid (RNA) in nucleoli and cytoplasm is well preserved. Technique: Fi in Carnoy's fluid (ethanol:acetic acid 3:1 or ethanol:chloroform:acetic acid 6:3:1) or in aldehydes (10% formalin or 2.5% glutaraldehyde bsered to pH 7.0). Hydrolyse deparaEnii sections 12-24 hr at 27-50 C in Bouin's fluid, wash in distilled water, immerse in 25% (v/v) acetic acid, treat 1 hr at 27-30 C with 10% (v/v) dine in 25% acetic acid, wash in 25% acetic acid and then in water. Stain 10-40 min with 0₃% toluidine blue in 0.05 M potassium biphthalate bder (pH 4.0); rinse in distilled water, pass to 10% (w/v) ammonium molybdate for 1 min, rinse again in water and pass through tert-butanol and xylene to a synthetic resin. Chromatin and chromosomes are pale green; RNA in nucleoli and cytoplasm deep purple.     

Chlorous Acid as An Agent for Blocking Tissue Aldehydes

Chlorous acid (HClO₂), which is known to convert aldehyde groups to carboxylic groups, was found to be an effective blocking agent for tissue aldehydes. A 0.2 M solution of NaClO₂ in 1 M acetic acid was found to block completely the Feulgen, PAS, ninhydrin-Schiff and plasmal reaction within 8 hr at 20 C. This blocking reaction appears to be irreversible.     

Histochemical Demonstration of Acid Phosphatase in Hard Tissues

The action of the following decalcifying solutions for the demonstration of acid phosphatase has been studied: buffer solution acetic-acetate 0.05 M, pH 5; 2, 5, 10, 20, and 50% formic acid and 20% sodium citrate in equal parts (pH 2.6, 3, 3.8, 4.2, and 5); 0.5 M citric acid-NaOH, pH 4.2; Versene solution, 5%, pH 7. A comparative study of fixatives has been made also (neutral formalin, 10-20%; formalin-chloral hydrate (Fishman), acetone and 80% alcohol). The best results were obtained with fixation at 4°C in 10-20% neutral formalin or formalin-chloral hydrate, for a period of 24 hr, and decalcification with 20% sodium citrate, 5% formic acid, in equal parts, pH 4.2, which can act on both specimens or sections for a period up to 2 wk with very little loss of enzyme. It is not necessary to reactivate the enzyme after decalcification; frozen sections should be used and should be washed in distilled water before proceeding with the demonstration of the enzyme (Gomori's method or azo dye coupling). Other fixatives (acetone and alcohol) and paraffin embedding produce a greater loss in enzymes and very irregular results.     

The Application of Miller's Elastic Stain to Glycol Methacrylate Tissue Sections

The application of Miller's dilute elastic stain followed sequentially by Gill's III hematoxylin and a fast green counterstain produced a reliable and consistent method for differentially staining elastic fibers, nuclei, muscle and collagen in glycol methacrylate tissue sections. Evaluation of different methods of fixation and conditions of staining on animal tissue sections showed that elastic fibers in both perfusion and immersion fixed tissues can be intensely stained. The stability of Miller's elastic stain offers the potential of a commercially available histological stain reagent for coarse and fine elastic fibers in glycol methacrylate tissue sections.