Categories: All - minerals - solution - advantage - procedure

by Sherlene Peter 4 years ago

725

INTRODUCTION TO FOOD ANALYSIS

Dry ashing involves incinerating samples at high temperatures using a muffle furnace, leading to the vaporization of water and other volatile materials, while organic substances are oxidized to CO2, H2O, and N2.

INTRODUCTION TO FOOD ANALYSIS

VITAMINS

THE INTENSITY OF THE BLUE FLUORESCENCE PROPORTIONAL TO THE THIAMINE CONCENTRATION. AND IT IS COMPARED WITH STANDARD SOLUTION.
THIOCHROME FLUOROMETRIC METHOD: THE MATERIAL TO BE EXAMINED MUST DIGESTED WITH SULFURIC ACID AND TREATED WITH A PHOSPHATASES PREPARATION. THE THIOCHROME RESULTING FROM OXIDATION WITH POTASSIUM FERRICYANIDE, HYDROGEN PEROXIDE IN ALKALINE SOLUTION IS EXTRACTED WITH ISOBUTYL ALCOHOL.

METHOD

DISADVANTAGE: TOXICITY OF CYNOGEN BROMIDE- THE ANALYSIS MUST BE CARRIED OUT UNDER FUME HOOD.
COLORIMETRIC METHOD: REACTION BETWEEN NIACIN(NICOTIC ACID AND CYNOGEN BROMIDE WILL FORMS COLOURED COMPOUND WITH AN INTENSITY PROPORTIONAL TO NIACIN CONCENTRATION.
FLUOROMETIC METHOD: THIS METHOD MEASURES BOTH ASCORBIC ACID AND DEHYDROASCORBIC ACID. ASCORBIC ACID OXIDIZED TO DEHYDROASCORBIC ACID UPON REACTION WITH O-PHENYLAMINE. THE REACTION WILL FORMED A FLUORESCENT QUINOXALINE COMPOUND. THE FLUOROSCENT COMPOUND= VIT. C CONTENT.
2,6-DICHLOROPHENOLINDOPHENOL TITRIMETRIC METHOD: L-ASCORBIC ACID IS OXIDIZES TO DEHYDROASCORBIC ACID BY INDICATOR DYE. IT MEASURES THE DECOLOURIZATION OF DYE BY ASCORBIC ACID. AT THE ENDPOINT, EXCESS OF UNREDUCED DYE IS ROSE PINK IN ACID SOLUTION LASTING AT LEAST 10 SEC.
DISADVANTAGE: THIS METHOD IS NOT SUITABLE FOR HIGHLY COLOURED PRODUCTS BECAUSE OF DIFFICULTY OF DETERMINING THE ENDPOINT DURING TITRATION.

METHODS

HPL METHOD- THIS METHOD INVOLVES CHROMATOGRAPHIC SEPARATION AND QUANTITATIVE DETERMINATION AT 325NM.
COLORIMETRIC METHODS- MEASURES THE UNSTABLE COLOUR AT A620NM THAT RESULTS FROM REACTION BETWEEN VIT A AND ANTIMONY TRICHLORIDE. BLUE COLOUR= AMOUNT OF RETINOL IN FOOD SAMPLE. THE COLOUR IS MEASURED AGAINST THE SE OF KNOWN STANDARDS.

ASH AND MINERALS

WET ASHING

Disadvantage: hazardous and used corrosive reagent.
Advantage: mineral stay in solution,little loss from mineral volatilization, rapid than dry ashing.
PRINCIPLE: Oxidation of organic substances by strong acid (HNO3) and oxidizing agent, perchloric acid (HClO4), Sample solution is heated up slowly up to 350 degree celsius until organic matter is completely digested (leaving only mineral oxides in solution) and HNO3 is almost evaporated, Boiling of sample solution is continued until the solution become colourless or light in colour, Solution is cooled, and 50% of HCl is added and diluted with distilled, deionized water.

DRY ASHING

DISADVANTAGE:Time consuming (12 – 18 hrs, or overnight) Loss of volatile elements at high temp. e.g. Cu, Fe, Pb, Hg, Ni, Zn, Interactions between mineral components and crucibles.
ADVANTAGE:Safe method,Requires no added reagents or blank subtraction. Large number of crucibles can be handled at once.Resultant ash can be used for other analyses e.g. acid insoluble ash, and water soluble and insoluble ash, Requires little attention, not labour intensive.
PRINCIPLE:. Incineration at high temp. with muffle furnace (5250 degree celcius or higher) ii. Water & other volatile materials are vaporized, organic substances are burned in the presence of the O2 in air to CO2, H2O and N2. iii.Most minerals are converted to oxides, sulfates, phosphates, chlorides or silicates. iv.The food sample is weighed before and after ashing to determine the concentration ash present.

LOW TEMPERATURE PLASMA DRY ASHING

Disadvantage: small capacity and the equipment is expensive.
ADVANTAGE:Less chances of losing trace elements by volatilization, Equipment of choice for volatile salts. Utilization of O2 as sole reagent.
PRINCIPLE: Sample is placed into a glass chamber, sealed and vacuum is applied. Small flow of O2 / air is introduced into the system while maintaining the specific minimum vacuum. Electromagnetic radio frequency generator is activated to control the rate of incineration, excites the gas molecules and dissociates it into chemically active atoms and molecules. Combustion products which are completely dissociated are carried away in the gas stream. Variable power frequency adjusts the rate of incineration.

ACID INSOLUBLE ASH

PROCEDURE: Ash is diluted with distilled water, then heated to nearly boiling, the resulting solution is filtered and washed several times with hot distilled water. Dry and re-ash the filter paper in muffle furnace at least 30 min. until constant weight is achieved. The weight remaining represents the amount of insoluble ash. Calculate soluble ash by subtracting insoluble ash from total ash, or, dry the filtrate, re-ash and weigh.

ALKALINITY OF ASH

PROCEDURE :Place ash (total / water-insoluble ash) in platinum dish. Add 0.1N HCl and warm on a steam bath. Cool and transfer to Erlenmeyer flask, titrate HCl with 0.1N NaOH using methyl orange as indicator. Express the result as mL of 1N acid / 100g sample.

DIETARY FIBER

ENGLYST-CUMMINGS METHOD

Advantage: suitable for determining fiber content in most foods(low content of ligning), it allow estimation of resistant starch.
Defatted food sample is heated in water. Enzymes are then added to precipitate fiber, which is separated from digest by centrifugation, then is washed & dried. Fiber is then hydrolyzed using concentrated sulfuric acid solution to break down into mono. Concentration of mono is determined colorimetrically or chromatographically. Mass of fiber in original sample assumed to be equal to the total mono present.

THEANDER-MARLETT METHOD

Advantage: suitable for research, legislation, and labeling purpose, provides most accurate estimate of fiber for wide range of food.
Principle: free sugars and lipids are extracted with ethanol and hexane. Starch is removed by enzymatic digestion & insoluble fiber is separated from soluble fiber. Fiber fractions are hydrolyzed with sulfuric acid and sugar content of the acid hydrolysates is determined. Lignin is determined gravimetrically.

ACID & ALKALI DIGESTION METHOD

Disadvantage: The method measures variable amounts of the celluloses and lignin in the sample, but hemicelluloses, pectins and hydrocolloids are solubilized and not detected.
Principle: Digestible CHO, lipids and protein are selectively solubilized by chemical and enzymes. Indigestible materials are then collected by filtration, and the fibre residue is quantitated gravimetrically. This method only measures celluloses and lignin.

AOAC METHOD

Advantage: The method can be used to determine fiber content in all foods Disadvantage: greatly overestimate he fiber content with a high content of simple sugars.
Principle: to isolate the fraction of interest by selective precipitation and then to determine its mass by weighing. Insoluble fiber is collected by filtration soluble fiber is precipitated by bringing the filtrate to 78% ethanol and collected by filtration.

CARBOHYDRATE

REFRACTIVE INDEX (RI) MEASUREMENT

Advantage: Method is quick & simple to carry out, gives direct reading and require only one or two drops of sample, performed with simple hand-held instrument.
Principle: RI(n) of a substance is the ratio of light velocity in a vacuum to its velocity of a substance. When electromagnetic radiation passes from one medium to another, it can change direction; RI of a material can be determined by measuring the ratio of angle of incidence.

POLARIMETRY

Principle: Asymmetric carbon atoms have the ability to rotate plane of polarization of polarized light. Plane polarized light passed through solution exhibiting optical activity, it rotated either to left(-) or right(+). Angle of polarization proportional to the concentration of optically active molecules in solution. Prior to analysis, sample solution must be clarified. CHO able rotate plane polarized light through an angle of rotation.
Disadvantage: Polarimetry method unable to analyzed mixtures of CHO(except sucrose in the presence of other CHO)

NELSON-SOMOGYI METHOD

Principle: The reducing sugar when heated with alkaline copper tartrate reduce the copper, from cupric to cuprous state, thus cuprous oxide is formed. Cuprous oxide is treated with arsenomolybdate. Reduction of arsenomolybdate complex produce an intense, stable blue-coloured solution. The absorbance of the solution is determined at either 500-520nm against standard

MUNSON-WALKER METHOD

Disadvantage: same disadvantage as Lane-Eynon method
Advantage: more reproducible and accurate
Principle: Involving oxidation of the CHO in the presence of heat and an excess of copper sulfate and alkaline tartrate under carefully controlled conditions-leads to the formation of a copper oxide precipitate. Amount of precipitate formed is directly related to the concentration of reducing sugar in the sample. Concentration of precipitate present can be determined through gravimetrically and titrimetrically.

LANE-EYNON METHOD

Disadvantage: The reaction is not stoichiometric- necessary to prepare a calibration curve with a series of standard solutions of known CHO concentration, result depends on the precise reaction time, temperature & reagent concentration), cannot distinguish between different types of reducing sugar.
Advantage: for determinations of reducing sugars in honey and other high reducing sugar syrups.
Principle: Based on the reaction of reducing sugar with a solution of copper sulfate followed by reaction with alkaline tartrate. The mixture is boiled for a specific time, followed by addition of methylene blue(as an indicator), coloured solution is titrated until decolouration of the indicator.

PROTEIN

KJEDAHL METHOD

Disadvantages: does not give a measure of the true protein- measures total organic nitrogen, different proteins need different correction factors, time consuming and use corrosive reagents.
Advantages: applicable to all types of food, relatively simple and inexpensive.
Principle: Proteins and other organic food components in a sample are digested with sulphuric acid in the presence of catalysis. Total organic Nitrogen is converted to ammonium sulfate; digest is neutralized with alkali and distilled into boric acid solution. Borate anions are formed & titrated with standardized acid- converted to nitrogen in the sample.

LOWRY METHOD

Disadvantage: colour varies with different protein to a greater extent than Biuret method, colour is not strictly proportional to protein concentration. The reaction is interfered with varying degrees of sucrose,lipids,monosaccharides and etc.
Advantages: very sensitive, less affected by turbidity of the sample, relatively simple
Principle: Lowry method combines Biuret reagent with another reagent (FOLIN-CIOCALTEAU PHENOL reagent) which reacts with tyrosine and trytophan residues in proteins. The reaction gives a bluish colour; the absorbance is read at 750nm( high sensitivity for low protein) 500nm( low sensitivity for high protein concentration)

DYE BINDING METHOD

Disadvantage: not sensitive; mg quantities of protein are required, proteins differ in basic amino acid content, so differ in dye-binding capacity, non-protein component bind dye until cause error.
Advantage: rapid, inexpensive, relatively accurate, no corrosive reagents,more precise than Kjedahl method, does not measure non-protein nitrogen.
Principle: Protein containing sample is mixed with a known excess amount of anionic(negatively charged) dye in a buffered solution; proteins bind to the dye, to form an insoluble complex(electrostatic attraction between the molecule), the amount of unbound soluble dye is determined by measuring its absorbance. Unbound dye is inversely related to the protein content of the sample.

BIURET METHOD

Disadvantages: relatively low sensitivity compared to other UV-vis methods, opalescence could occur in the final solution with presence of high levels of lipids and carbohydrates.
Advantages: rapid test(analysis can be completed within 30 minutes), does not detect nitrogen from non-peptide or non-protein source.
Principle: Biuret method involves a reaction with peptide linkages,cupric ions complexed with peptide bonds-under alkaline conditions and produced a violet-purplish colour. Absorbance of the colour produced is read at 540nm. The colour intensity(absorbance) is proportional to the protein content of the sample.

CRUDE FAT

NON- WET SOLVENT EXTRACTION METHOD

DETERGENT METHOD
Principle: Detergent react with protein to form a protein- detergent complex to break up emulsions & release fat, milk is pipetted into a Babcock test bottle. An anionic detergent(dioctyl sodium phosphate) is added to disperse the protein layer that stabilizes the fat and also liberate the fat. Strong hydrohphilic non-ionic polyoxyethylene detergent sorbitan monolaurate is added to separate fat from other food component.

Advantage: does not used corrosive reagent like in Babcock Method

GERBER METHOD FOR MILK FAT
Principle: Sulphuric acid is added to a known amount of milk in Gerber tube or butyrometer for digestion of protein and carbohydrates- it also help to release fats and maintains the fat in liquid state by generating heat. The amyl alcohol is added into the mixture to give a clear, homogeneous fat column and the tube is carefully inverted and centrifuged and incubated in waterbath at 60-63 degree Celsius fro 5 min.

ADVANTAGE: wider application to a variety of dairy products, it much simpler and faster because isoamyl alcohol generally improves the fat separation and reduces the effect of sulfuric acid and also prevent the charring of sugar.

BABCOCK METHOD FOR MILK FAT
Principle: Sulphuric acid is added to a known amount of milk in Babcock bottle. The mixture is shaken until homogeneous,centrifuged and submerged into water at 63 degree Celsius. Subsequently centrifugation and addition of hot water isolate fat for quantification in the graduated portion of test bottle.

ADVANTAGE: for modified Babcock method it can be used to determine essential oil in flavour extracts and fat in seafood. DISADVANTAGE: it does not determine phospholipids in the milk products and not applicable to product containing chocolate or sugars.

WET SOLVENT EXTRACTION METHOD

MOJONNIER METHOD
Principle: Fat is extracted with a mixture of ethyl ether and petroleum-ether in a Mojonnier flask. The extracted fat is dried to a constant weight and expressed as percent(%) fat by weight.

ADVANTAGE: does not require prior removal of moisture from sample, extraction are repeated three times DISADVANTAGE: use many chemical reagents during the extraction process.

SOXHLET METHOD
Principle: Thimble(containing the sample) is placed in an extraction chamber, which suspended above a flask containing the solvent & below the condenser. The flask is heated, the solvent evaporates & moves up into the condenser and converted into a liquid & drips back into the extraction chamber containing sample.

ADVANTAGE: provides soaking effect of the sample(provide more complete extraction of fat from the sample), avoid channeling of the solvent. DISADVANTAGE: the extraction took a long time(4 hours- 16 hours)

GOLDFISCH METHOD
Principle: Sample is put in an extraction ceramic thimble and the solvent is added into the boiling flask. The sample must ground to small particle size prior to analysis. Method allows the solvent from boiling flask to continuously flows over the sample that held in a ceramic thimble.

ADVANTAGE: faster and more efficient extraction method than Soxhlet extraction method. DISADVANTAGE: channeling of the solvent may occur inefficient/ incomplete extraction.

MOISTURE

CHEMICAL METHOD- KARL-FISCHER TITRATION

PRINCIPLE: Karl-Fischer reagent is added directly as the titrant if the water in the sample is accessible, if the moisture is inaccessible to the reagent, the moisture is extracted from the food with an appropriate solvent. A KFR water equivalent must be determined, iodine and SO2 in the appropriate form are added to the sample in a closed chamber protected from atmospheric moisture. The end point colour is dark-brown.
ADVANTAGES: suitable for low-moisture foods that are sensitive to decomposition/ volatilization under vaccum or high temperature. DISADVANTAGES: incomplete water extraction due to atmospheric condition, moisture adhering to the walls of unit, interferences from certain food constituents.

DISTILLATION METHOD

PRINCIPLE: involves co-distilling the water in a food sample with a high boiling point solvent that is immiscible in water, the distilled water is condensed. collecting the mixture that distills off in a collecting vessel or trap- measuring the volume of H20
DIRECT DISTILLATION(DEAN AND STARK) OR REFLUX DISTILLATION

ADVANTAGES: suitable for application to foods with low- moisture contents, application to food containing volatile oils, equipment is relatively cheap, easy to setup and operate. DISADVANTAGES: destructive, relatively time-consuming, involving the use of flammable solvents, not applicable to some types of food.

OVEN DRYING METHOD

PRINCIPLE: The sample is heated under specified conditions until constant weight, and calculation of moisture is based on loss of weight and the thermal energy is used to evaporate the water from the food sample
ADVANTAGES: precise,relatively cheap,easy to use officially approved for many samples can be analyzed. DISADVANTAGES: destructive, unsuitable for some types of food and time consuming

FOOD ANALYSIS

EVALUATION OF ANALYTICAL DATA

Repeatability: where the test results are obtained with the same method on identical test items in the same lab by the same operator within short interval time.
Reproducibility: where the test results are obtained with the same method on identical test items in different lab with different operators using different equipments.

dffg

Precision: how close replicate measures are indicates reproducibility
Specificity: of a particular analytical method (how well the method detects & measures the compound of interest)
Accuracy: how close the experimental measure is to the correct/true value of an analyzed substance
Sensitivity: relates to the magnitude of changes of measuring devices(instruments)

SAMPLE PRESERVATION

sample should be stored under conditions that prevent degradation
to prevent changes in food composition and degradation

SAMPLE PREPARATION

at least performed 3 times(triplicate)
analysis requires reduction in amount from the total population & simultaneously reduction of particle size
depend on nature of food