AOAC 985.29 食物中总膳食纤维 酶-重量法

更新时间:2023-06-28 11:38:31 阅读: 评论:0

45.4.07
AOAC Of f i c ial Method 985.29
To t al Di e tary Fi b er in Foods
Enzymatic–Gravimetric Method
First Ac t ion 1985适合发说说的句子
Fi nal Ac tion1986
AOAC–AACC Method
Co d ex-Adopted–AOAC Method*
A.Prin ci ple
Du p li c ate test por t ions of dried foods, fat-extracted if con t ain i ng >10% fat, are gelatinized with Termamyl (heat-stable α-am y l a), and then en z y m at i c ally di g ested with pro t e a and amyloglucosida to re m ove pro t ein and starch. (When an a l yz i ng mixed di e ts, al w ays ex t ract
fat prior to de t er m in i ng to t al di e tary fi b er.) Four vol u mes of ethyl al c o h ol are added to pre c ip i t ate sol u b le di e tary fi b er. To t al res i d ue is fil t ered, washed with 78% ethyl al c o h ol, 95% ethyl al c o h ol, and ac e t one. Af t er dry i ng, res i d ue is weighed. One du p li c ate is an a l yzed for pro t ein, and other is in c in e r a ted at 525°C and ash is de t er m ined. To t al di e tary fi b er = weight res i d ue – weight (pro t ein + ash).
B. Ap p a r a t us
(a)Fritted cru c i b le.—Po r os i ty No. 2 (Py r ex No. 32940, coar, ASTM 40-60 µm; or Corning No. 36060 Büchner, fritted disk, Py r ex, 60 mL, ASTM 40-60 µm). Clean thor o ughly, heat 1 h at 525°C, and soak and then rin in H2O. Add ca 0.5 g Celite to air-dried cru c i b les and dry at 130°C to con s tant weight (≥ 1 h). Cool and store in des i c c a t or un t il ud.
(b) V ac u um source.—V ac u um pump or as p i r a t or equipped with in-line dou b le vac u um flask to pre v ent con t am i n a t ion in ca of H2O backup.
(c) Vac u um oven.—70°C.Al ter na tively,105°C air oven can be ud.
(d) Des ic ca tor.
最恐怖的恐怖片(e)Muf fle fur nace.
(f)Wa t e r b a t h s.—(1)B o i l i n g.(2)C o n s t a n t tem p er a t ure.—Ad j ust a ble to 60°C, with ei t her multistation shaker or multistation mag n etic stir r er to pro v ide con s tant ag i t a t ion of di g es t ion flasks dur i ng en z y m atic hy d ro l y s is.
(g) Beakers.—Tall-form, 400 or 600 mL.
(h) Bal a nce.—An a lyt i cal,readability to0.1mg.
(i)pH me t er.—Stan d ard i zed with pH 7 and pH 4 buff e rs.
C. Re a gents
(a) 95% Eth a n ol.—v/v. Technical grade.
(b) 78% Eth a n ol.—Place 207 mL H2O into 1 L vol u m et r ic flask. Di l ute to vol u me with 95% ethyl al c o h ol. Mix and di l ute to vol u me again with 95% ethyl al c o h ol if nec e s s ary. Mix. One vol u me H2O mixed with 4 vol u mes 95% ethyl al c o h ol will also give 78% ethyl al c o h ol fi n al con c en t ra t ion.
(c)Ac e tone.
(d)Phos p hate buffer.—0.08M, pH 6.0. Dis s olve 1.400 g so d ium phos p hate dibasic, an h y d rous (Na2HPO4) (or 1.753 g dihydrate) and 9.68 g so d ium phos p hate monobasic monohydrate (NaH2PO4⋅H2O) (or 10.94 g dihydrate) in ca 700 mL H2O. Di l ute to 1 L with H2O. Check pH with pH me t er.
(e) Al p ha-amyla (heat sta b le).—Termamyl. (1) Store in re frig er a tor.Bad on Nel s on/Somogyi re d uc i ng sugar with sol u b le starch as sub s trate.—10 000 + 1000 units/mL (1 unit is de f ined as the amount of en z yme re q uired to re l ea 1 µmole re d uc i ng sugar equiv a l ents/min at pH 6.5 and 40°C). (2) Bad on Ceralpha method us i ng p-nitrophenyl-maltosaccharide as sub s trate in the pres e nce of a thermostable al p ha-glucosida.—3000 + 300 Ceralpha units/mL (1 unit of en z yme is re q uired to re l ea 1 µmole p-nitrophenyl/min at pH 6.5 and 40°C).
(f) Pro te a.—Keep re frig er ated.(1)Ca in as say.—300–400 Units/mL. (1 pro t e a unit is de f ined as the amount of en z yme re q uired to hy d ro l yze (and solubilize in TCA) 1 µmole ty ro sine equiv a l ents/min from sol u b le ca s ein at pH 8.0 and 40°C); 7–15 units/mg (1 unit will hy d ro l yze ca s ein to pro d uce color equiv a l ent to 1.0 µmole ty r o s ine/min at pH 7.5 and 37°C). Color by F
olin-Ciocalteau re a gent. (2) Azo-cain as s ay.—300–400 Units/mL [1 unit endo-peptida ac t iv i ty is de f ined as the amount of en z yme re q uired to hy d ro l yze (and solubilize in TCA) 1 µmole ty r o s ine equiv a l ents/min from sol u b le ca s ein at pH 8.0 and 40°C].
(g) Amyloglucosida.—Keep re frig er ated.(1)Starch/glu c o oxida–peroxida method.—2000–3300 Units/mL (1 unit en z yme ac t iv i ty is de f ined as the amount of en z yme re q uired to re lea1µmole glu c o/min at pH 4.5 and 40°C). (2) PNPBM (p-nitrophenyl beta-maltosida) method.—130–200 Units/mL (1 unit en z yme ac t iv i ty [PNP unit] is the amount of en z yme, which in the pres e nce of ex c ess lev e ls of beta-glucosida, will re l ea 1 µmole p-nitrophenyl from p-nitrophenyl beta-maltosida/min at 40°C).
The only en z yme which has been found to be sig n if i c antly con tam i nated with in ter fer ing ac tiv i ties is amyloglucosida. Thermostable al p ha-amyla and pro t e a from com m er c ial sources have been found to be gen e r a lly free of in t er f er i ng en z ymes. Low lev e ls of beta-glucana have been de t ected in pro t e a prep a r a t ions, but at lev e ls well be l ow that which would in t er f ere with to tal di etary fi ber anal y sis.The ma jor con tam i nant in amyloglucosida prep a r a t ion was shown to be an endo-cellula and re s ulted in endo-depolymerization of mixed-linkage beta-glucan from bar l ey and oats, with re s ul t ant un d er e s t i m a t ion of this di etary fi b2022年冬奥会吉祥物
er com po nent.The con tam i na tion of amylogucosida with endo-cellula (beta-glucana) can be eas ily de tected.
Al t er n a t ively, there are kits con t ain i ng all 3 en z ymes (pre t ested) avail a ble from a num b er of com p a n ies.
(h)So dium hy drox ide so lu tion.—0.275M. Dis s olve 11.00 g NaOH ACS in ca 700 mL H2O in 1 L vol u m et r ic flask. Di l ute to vol u me with H2O.
(i) Hy d ro c hlo r ic acid so l u t ion.—0.325M. Di l ute stock so l u t ion of known ti t er, e.g., 325 mL 1M HCl, to 1 L with H2O.
(j) Celite.—Acid-washed.
用激动造句© 2005 AOAC IN T ER N A T IONAL Ta b le 985.29. Test sam p les for en z yme pu r ity
Test sam p le
脚底发热Ac tiv ity
tested
Test por t ion
weight, g
Ex pected
re cov ery,% Cit rus pec tin Pectina0.195–100 Stractan (larch gum)Hemicellula0.195–100 Wheat starch Am y la  1.00–1
Corn starch Am y la  1.00–2
Ca in Pro te a0.30–2
β-Glucan (bar l ey gum)aβ-Glucana0.195–100
a
Sigma Chem i c al Co. or Megazyme In t er n a t ional Ire l and, Ltd.
D.En zyme Pu rity
形容感情好的成语
To en sure ab nce of un de sir able en zy matic ac tiv ity in en zymes ud in this pro c e d ure, run ma t e r i a ls listed in Ta b le 985.29 through en t ire pro c e d ure each time lot of en z ymes is changed, or at max i m um in t er v al of 6 months to en s ure that en z ymes have not de g raded.
E. Test Por t ion Prep a r a t ion
De t er m ine to t al di e tary fi b er on dried test sam p le. Ho m og e n ize test sam p le and dry over n ight in 70°C vac u um oven, cool in des i c c a t or, and dry-mill test sam p le to 0.3–0.5 mm mesh. If test sam p le can n ot be heated, freeze-dry be f ore mill i ng. If high fat con t ent (>10%) pre v ents proper mill i ng, defat with pe t ro l eum ether (3 times with 25 mL por t ions/g test sam p le) be f ore mill i ng. Re c ord loss of weight due to fat re m oval and make ap p ro p ri a te cor r ec t ion to fi n al % di e tary fi b er found in de t er m i n a t ion. Store dry-milled test sam p le in capped jar in des i c c a t or un t il anal y s is is car r ied out.
F.De ter mi na tion
Run blank through en t ire pro c e d ure along with test por t ions to mea s ure any con t ri b u t ion from re a gents to res i d ue.
Weigh du p li c ate 1 g test por t ions, ac c u r ate to 0.1 mg, into 400 mL tall-form beak e rs. Test por t ion weights should not dif f er >20 mg. Add 50 mL pH 6.0 phos p hate buffer to each beaker. Check pH and ad j ust to pH 6.0 ± 0.2 if nec e s s ary. Add 0.1 mL Termamyl so l u t ion. Cover beaker with Al foil and place in boil i ng water bath 15 min. Shake gently at 5 min in t er v als. In c rea in c u b a t ion time when num b er of beak e rs in boil i ng water bath makes it dif f i c ult for beaker con tents to reach in ter nal tem per a ture of95°–100°C. U ther mom e ter to in di cate that 15 min at 95°–100°C is at t ained. To t al of 30 min in water bath should be suf f i c ient.
Cool so l u t ions to room tem p er a t ure. Ad j ust to pH 7.5 ± 0.2 by add i ng 10 mL 0.275M NaOH so l u t ion.
缥缈的反义词Add 5 mg pro t e a . (Pro t e a sticks to spat u la, so it may be pref e r a b le to pre p are en z yme so l u t ion (50 mg in 1 mL phosphate buffer) and pipet 0.1 mL to each sam p le just be f ore u.
Cover beaker with Al foil. In c u b ate 30 min at 60°C with con t in u o us ag i t a t ion. Cool. Add 10 mL 0.325M HCl so l u t ion. Mea s ure pH and dropwi add acid if nec e s s ary. Fi n al pH should be 4.0–4.6. Add 0.3 mL amyloglucosida, cover with Al foil, and in c u b ate 30 min at 60°C with con
tin u ous ag i ta tion.Add280mL 95% ethyl al c o h ol pre h eated to 60°C (mea s ure vol u me be f ore heat i ng). Let pre c ip i t ate form at room tem p er a t ure for 60 min. Weigh cru c i b le con t ain i ng Celite to near e st 0.1 mg, then wet and re d is t rib u te bed of Celite in cru c i b le by us i ng stream of 78% ethyl al c o h ol from wash bot t le. Ap p ly suc t ion to draw Celite onto fritted glass as even mat. Main t ain suc t ion and quan t i t a t ively trans f er pre cip i tate from en zyme di gest to cru ci ble.
Wash res i d ue suc c es s ively with three 20 mL por t ions of 78% ethyl al c o h ol, two 10 mL por t ions of 95% ethyl al c o h ol, and two 10 mL por t ions of ac e t one. Gum may form with some prod u cts, trap p ing liq u id. If so, break sur f ace film with spat u la to im p rove fil t ra t ion. Time for fil t ra t ion and wash i ng will vary from 0.1 to 6 h, av e r a g i ng 0.5 h per sam p le. Long fil t ra t ion times can be avoided by care ful in ter mit tent suc tion through out fil tra tion.
Dry cru c i b le con t ain i ng res i d ue over n ight in 70°C vac u um oven or 105°C air oven. Cool in des i c c a t or and weigh to near e st 0.1 mg. Sub t ract cru c i b le and Celite weight to de t er m ine weight of res i d ue. An a l yze res i d ue from 1 test por t ion of t of du p li c ates for pro t ein by 960.52 (e 12.1.07), us i ng N × 6.25 as con v er s ion fac t or, ex c ept in cas where N con t ent in pro t ein is known.
In c in e r a te c o nd test por t ion of du p li c ate 5 h at 525°C. Cool in des i c c a t or and weigh to near e st 0.1 mg. Sub t ract cru c i b le and Celite weight to de t er m ine ash.
G.Cal cu la tions
De t er m i n a t ion of blank:
杀龙
B = blank, mg = weight res i d ue − P B−A B
where weight res i d ue = av e r a ge of res i d ue weights (mg) for du p li c ate blank de t er m i n a t ions; and P B and A B = weights (mg) of pro t ein and ash, re s pec t ively, de t er m ined in first and c o nd blank res i d ues.
Cal c u l ate TDF as fol l ows:
TDF, % =
[(weight res i d ue −P−A−B) / weight test por t ion] × 100 where weight res i d ue = av e r a ge of weights (mg) for du p li c ate blank de t er m i n a t ions; and P and A = weights (mg) of pro t ein and ash, re s pec t ively, in first and c o nd test por t ion res i d ues; and weight test por t ion = av e r a ge of 2 test por t ion weights (mg) taken.
Ref er ences:JAOAC 68, 677(1985); 69, 259(1986).
Re v id: June 2003
*  Adopted as a Co d ex De f ining Method for gravimetry/en z y m atic di g est of to t al di e tary fi b re in spe c ial foods.
© 2005 AOAC IN T ER N A T IONAL

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