Filters freeze drying

Into a 1-litre beaker, provided with a mechanical stirrer, place 36 - 8 g. (36 ml.) of aniline, 50 g. of sodium bicarbonate and 350 ml. of water cool to 12-15° by the addition of a little crushed ice. Stir the mixture, and introduce 85 g. of powdered, resublimed iodine in portions of 5-6 g, at intervals of 2-3 minutes so that all the iodine is added during 30 minutes. Continue stirring for 20-30 minutes, by which time the colour of the free iodine in the solution has practically disappeared and the reaction is complete. Filter the crude p-iodoaniline with suction on a Buchner funnel, drain as completely as possible, and dry it in the air. Save the filtrate for the recovery of the iodine (1). Place the crude product in a 750 ml. round-bottomed flask fitted with a reflux double surface condenser add 325 ml. of light petroleum, b.p. 60-80°, and heat in a water bath maintained at 75-80°. Shake the flask frequently and after about 15 minutes, slowly decant the clear hot solution into a beaker set in a freezing mixture of ice and salt, and stir constantly. The p-iodoaniline crystallises almost immediately in almost colourless needles filter and dry the crystals in the air. Return the filtrate to the flask for use in a second extraction as before (2). The yield of p-iodoaniline, m.p. 62-63°, is 60 g. 

Dimethylhexane-2,5-diol [110-03-2] M 146.2, m 88-90. Purified by fractional crystn. Then the diol was dissolved in hot acetone, treated with activated charcoal, and filtered while hot. The soln was cooled and the diol was filtered off and washed well with cold acetone. The crystn process was repeated several times and the crystals were dried under a vac in a freeze-drying apparatus [Goates et al. J Chem Soc, Faraday Trans 1 78 3045 1982]. 

Sodium poly(a-L-glutamate). It was washed with acetone, dried, dissolved in water and ppted with isopropanol at 5°. Impurities and low molecular weight fractions were removed by dialysis of the aqueous solution for 50h, followed by ultrafiltration through a filter impermeable to polymers of molecular weights greater the 10. The polymer was recovered by freeze-drying. [Mori et al. J Chem Soc, Faraday Trans I 2583 1978.]... 

Five parts of the terpene, 7 of amyl nitrite, and 12 of glacial acetic acid are mixed and cooled with ice and salt, and a mixture of 6 parts of hydrochloric acid and 6 parts of glacial acetic acid added in small quantities at a time. Five parts of alcohol are then added and the mixture allowed to stand in a freezing mixture for a itime. A mass of crystals separates, which consists of the crude nitrosochlorides. This is filtered off and washed with alcohol. When perfectly dry 100 grams of the crystals are digested with 200 c.c. of chloroform for a few moments and at once filtered. The chloroform dissolves a-nitrosochloride, which is precipitated by the addition of excess of methyl alcohol. The crude compound is filtered off, dried and digested with anhydrous ether for... 

Thienylacetarnidocephalosporanic acid (7.0 g) was suspended in water (60 ml) and stirred with pyridine (7 ml) until the acid dissolved. The resulting solution (pH 5.9) was kept at 35°C for 3 days, then filtered and extracted with methylene chloride (4 x 60 ml). The methylene chloride extract was back-axtracted with a little water and the total aqueous solutions were then percolated through a column of Dowex 1x8 resin, (100 to 200 mesh, 150 g) in the acetate form at pH 4.3. The column was washed with water until the optical rotation of the eluate fell to zero and the eluate (500 ml) was freeze-dried. The residual white solid was dissolved in the minimum volume of methanol and after a few minutes the pyridine derivative crystallized this is the cephaloridine product. 

The solvent was evaporated off under reduced pressure, and the residual gum refluxed with concentrated hydrochloric acid (50 g) for 6 hours. The solution was aliowed to cool overnight. It was filtered from the phthalic acid crystals, and freeze-dried, and to the pink residue was added acetone (160 g) and ethyl acetate (50 g). The mixture was left in the cold room overnight and the clear pink supernatant liquid poured off. The pink gummy hydrochloride remaining in the flask was dissolved in water (20 g), saturated sodium acetate solution added until precipitation was complete, and the product collected and dried in a desiccator. The crude p-bis-(2-chloroethyl)-aminophenylalanine (3.6 g) was crystallized from methanol giving colorless needles, MP 172° to 174°C (decomp.) of p-bis-(2-chloroethyl)-aminophenylalanine. 

Bj Pivaloyloxymethyl D(—)-Ot-aminobenzylpenicillinate. hydrochloride To a solution of pivaloyloxymethyl D(—)-a-azidobenzylpenicillinate (prepared as described above) in ethyl acetate (75 ml) a 0.2 M phosphate buffer (pH 2.2) (75 ml) and 10% palladium on carbon catalyst (4 g) were added, and the mixture was shaken in a hydrogen atmosphere for 2 hours at room temperature. The catalyst was filtered off, washed with ethyl acetate (25 ml) and phosphate buffer (25 ml), and the phases of the filtrate were separated. The aqueous phase was washed with ether, neutralized (pH 6.5 to 7.0) with aqueoussodium bicarbonate, and extracted with ethyl acetate (2 X 75 ml). To the combined extracts, water (75 ml) was added, and the pH adjusted to 25 with 1 N hydrochloric acid. The aqueous layer was separated, the organic phase extracted with water (25 ml), and the combined extracts were washed with ether, and freeze-dried. The desired compound was obtained as a colorless, amorphous powder. 

Stir with 1000ml 50mM CDTA at pH 6.5 for 6h at 20-22X. Filter on G3 glass filter, wash residue with water, centrifuge filtrate at SOOOrpm for 20min, dialyse, concentrate. Reextract the residue under the same conditions and freeze-dry the combined filtrates CDTA-Fraction... 

In the first example, procaine penicillin, an aqueous vehicle containing the soluble components (such as lecithin, sodium citrate, povidone, and polyoxyethylene sorbitan monooleate) is filtered through a 0.22 pm membrane filter, heat sterilized, and transferred into a presterilized mixing-filling tank. The sterile antibiotic powder, which has previously been produced by freeze-drying, sterile crystallization, or spray-drying, is aseptically added to the sterile solution while mixing. After all tests have been completed on the bulk formulation, it is aseptically filled. 

Insensitive to impact, it decomposes, sometimes explosively, above its m.p. [1], particularly if heated rapidly [2], Although used in aqueous solutions as a preservative in pharmaceutical preparations, application of freeze-drying techniques to such solutions has led to problems arising from volatilisation of traces of hydrazoic acid from non-neutral solutions, condensation in metal lines, traps or filters, and formation of heavy metal azides in contact with lead, copper or zinc components in the drying plant [3,4],... 

Native factor VIII is traditionally purified from blood donations first screened for evidence of the presence of viruses such as hepatitis B and HIV. A variety of fractionation procedures (initially mainly precipitation procedures) have been used to produce a factor VIII product. The final product is filter-sterilized and filled into its finished product containers. The product is then freeze-dried and the containers are subsequently sealed under vacuum, or are flushed with an inert gas (e.g. N2) before sealing. No preservative is added. The freeze-dried product is then stored below 8 °C until shortly before its use. 

Packets of instant coffee proudly proclaim that the product has been freeze-dried . In practice, beans of coffee are ground, boiled in water and filtered to remove the depleted grounds. This process yields conventional fresh coffee, as characterized by its usual colour and attractive smell. Finally, water is removed from the coffee solution to prepare granules of instant coffee. 

Negative atmospheric pressure chemical ionization (APC) low-energy collision activation mss spectrometry has also been employed for the characterization of flavonoids in extracts of fresh herbs. Besides the separation, quantitative determination and identification of flavonoids, the objective of the study was the comparison of the efficacy of the various detection systems in the analysis of flavonoids in herb extracts. Freeze-dried herbs (0.5g of chives, cress, dill, lovage, mint, oregano, parsley, rosemary, tarragon and thyme) were ground and extracted with 20 ml of 62.5 per cent aqueous methanol. After sedimentation the suspension was filtered and used for HPLC analyses. Separations were carried out in an... 

The migration order of wine anthocyanins in CE has been studied in detail and the results have been compared with those obtained by RP-HPLC-MS. Wines were filtered and used for the analyses without any other pretreatment. Wine samples of 10 ml were freeze-dried, redissolved in methanol and applied for semi-preparative fractionation. CZE measurements were carried out in a fused-silica capillary (46 cm effective length, 75 /an i.d.). The capillary was conditioned with 0.1 M NaOH (2 min), water (2 min) and running buffer (5 min). The buffer consisted of 50 mM sodium teraborate (pH = 8.4) containing 15 per cent (v/v)... 

NMR analysis, the PHA was extracted from freeze-dried cells. For this purpose, 1.0 g freeze-dried cells were stirred in 200 mL of chloroform for 24 hours at 30°C. The extract was filtered to remove cells debris, and the chloroform was concentrated to a volume of about 15 ruL using rotary evaporator. The concentrated solution was then added drop-wise to 150 luL of rapidly stirred methanol to precipitate the dissolved PHA.The precipitated PHA was then recovered by filtration using a 0.45 pm PTFE membrane and dried overnight at room temperature. The purified PHA was dissolved in deuterated chlorofonn (CDCl ) and subjected to H and NMR analyses. 

Preparation of Aqueous Extract of Cotton Dust. Cotton cardroom dust was collected from V-cell filters in a commercial textile mill. A typical extraction was carried out by manually kneading 50 g of dust with 500 ml of deionized water for 5 min at 25°c and removing the liquor by centrifugation. The process was repeated twice with 250 ml of deionized water each time. The combined supernatant was filtered through filter paper by gravity and the filtrate (of final pH 8.3 without addition of buffer) was freeze-dried to yield fraction 1 (f-1). The major portion of f-1... 

Preparation of Aqueous Extract of Cotton Bract. Field-dried cotton bract, 10 g, picked directly from plants in a field near Lake Providence, Louisiana, was ground with mortar and pestle, extracted twice with 100 ml of deionized water at pH 7 for 30 min each time at 250c with stirring. The extracts were combined and the solution was filtered the filtrate was freeze-dried. This bract extract (bAg) was also used to immunize rabbits. Additional bAg was further purified by treatment with 85% methanol in a similar manner as with cotton dust. 

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