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Isolation, Purification, and Assay of
  Wheat Germ Acid Phosphatase
            Natalia Manzano
            Wilmarie Morales
             RISE Program
             May 10th, 2012
Objectives:
• To purify and isolate acid phosphatase
  from wheat germ.
• Determine protein concentration using
  Bicinchoninic Acid protein assay.
Introduction
• Wheat germ is a very small part of a wheat
  kernel.
• Wheat germ is very high in protein.
• It contains around 28% protein and has more
  protein than can be found in most meat
  products.
Wheat Germ Acid Phosphatase
  Catalyzes the hydrolysis of phosphate groups from
  macromolecules and smaller molecules that are stored in the
  wheat seed. The growing wheat embryo uses the freed
  phosphate in germination and growth.
Materials and Methods
Materials
25 g Wheat germ        MnCl2, 1.0 M               Centrifuge, high   Balance
H2O, prechilled to 4˚C Sodium acetate             speed
                       buffer, 1.0M (pH 5.7)      Ice bucket         Spectrophotomet
Cheesecloth            (NH4)2SO4, saturated                          er, visible
                       (pH 5.5)                   Magnetic stirrer   Microplate
Ice, crushed           Pasteur Pipets             Waterbaths (30˚C
                                                  and 70˚C)
BCA Kit                Gloves, disposable
BSA standard, 1.0      Weighing trays
mg/ml


Methods
               Bicinchoninic Acid protein assay
               (BCA)
               SDS PAGE
Procedure I: Obtaining Fractions
                                       Filter wheat germ
* All centrifugation was done at       with cheese cloth
              2800Xg
         at 4° for 20min
                                     Centrifuge filtrate (70ml)


Discard Pellet                                                                Fraction I

                                   Pellet                         Add 1.26 ml of MnCl2 1.0M
         Discard Pellet     Add Sodium Acetate                            Centrifuge
                                Centrifuge                            Supernatant 62 ml

                               Supernatant 25 ml                           Fraction II

                                   Fraction III
Pellet (buffer)                        Add 33.48 ml of Ammonium Sulfate
       Centrifuge                                     (Saturated 35%)
                                                     Supernatant 92 ml
                                                         Centrifuge
Discard Pellet
                                                       Add 46.92 ml of
                   Supernatant                       Ammonium Sulfate
                      21 ml                            (Saturated 57%)
                                                          Centrifuge
                                                     Supernatant 136 ml
                    Fraction IV
      Pellet                                             Fraction V
 Suspend in dH2O
    Centrifuge


                                  Fraction
Discard Pellet                       VI
Procedure II:   • BCA serves the purpose of
BCA Assay         reacting with complexes
                  between copper ions and
                  peptide bonds to produce a
                  purple end product.

                • Estimate visually or measure
                  with a standard
                  spectrophotometer or plate
                  reader (562nm).
Add Sample+
dH2O+BCA
Procedure III: SDS-PAGE
• Running Gel:                    • Stacking Gel:
  –   1.88 ml dH2O                   –   2.975 ml dH2O
  –   1.67 ml separating buffer      –   1.25 ml separating buffer
  –   2.22 ml Acrylamide             –   0.662 ml Acrylamide
  –   50.0 µl 20% SDS                –   225.0 µl 20% SDS
  –   100 µl 10% Glycerol            –   25 µl 10% Glycerol
  –   1.67 µl TEMED                  –   6.25 µl TEMED
  –   50 µl APS(100 mg/ml)           –   25 µl APS
Get sample obtained
                                              from previous purifying
                                              technique


                           Load Buffer
Set up gel, remove
comb




                                                 Load Sample (3:1
                                                  sample:buffer)
                           Run Gel



Stain with Coomassie and
Study Gel
                                     Procedure III: SDS
Results:
      Sample           Absorbance   Blank    Abs-Blank   Conc. (mg/ml)   Vol. of sample added   Dilution factor
  Fraction I 1X-L        2.511      0.094      2.417        25.466              2.3                    1
  Fraction I 1X-H        3.029      0.094      2.935        6.185               11.5                   1
 Fraction I X/10-L       0.305      0.094      0.211        22.231              2.3                   10
 Fraction I X/10-H       1.171      0.094      1.077        22.695              11.5                  10
Fraction I X/100-L       0.13       0.094      0.036        37.930              2.3                  100
Fraction I X/100-H       0.241      0.094      0.147        30.976              11.5                 100
  Fraction II 1X-L       3.029      0.094      2.935        30.923               2.3                   1
   Fraction II 1X-H      3.029      0.094      2.935        6.185               11.5                   1
  Fraction II X/10-L     0.385      0.094      0.291        30.660              2.3                   10
 Fraction II X/10-H      1.636      0.094      1.542        32.493              11.5                  10
 Fraction II X/100-L     0.164      0.094      0.07         73.752              2.3                  100
Fraction II X/100-H      0.512      0.094      0.418        88.081              11.5                 100
   Fraction III 1X-L     0.524      0.094      0.43         4.530               2.3                    1
   Fraction III 1X-H     2.035      0.094      1.941        4.090               11.5                   1
 Fraction III X/10-L     0.143      0.094      0.049        5.163               2.3                   10
 Fraction III X/10-H     0.317      0.094      0.223        4.699               11.5                  10
Fraction III X/100-L     0.094      0.094        0          0.000               2.3                  100
Fraction III X/100-H     0.138      0.094      0.044        9.272               11.5                 100
 Fraction IV 1X-L        0.536      0.094      0.442        4.657                2.3                   1
  Fraction IV 1X-H       1.541      0.094      1.447        3.049               11.5                   1
 Fraction IV X/10-L      0.149      0.094      0.055        5.795               2.3                   10
 Fraction IV X/10-H      0.303      0.094      0.209        4.404               11.5                  10
Fraction IV X/100-L      0.102      0.094      0.008        8.429               2.3                  100
Fraction IV X/100-H      0.163      0.094      0.069        14.540              11.5                 100
  Fraction V 1X-L        2.373      0.094      2.279        24.012               2.3                   1
  Fraction V 1X-H        3.029      0.094      2.935        6.185               11.5                   1
 Fraction V X/10-L       0.179      0.094      0.085        8.956               2.3                   10
 Fraction V X/10-H       0.673      0.094      0.579        12.201              11.5                  10
Fraction V X/100-L       0.151      0.094      0.057        60.055              2.3                  100
Fraction V X/100-H       0.358      0.094      0.264        55.630              11.5                 100
 Fraction VI 1X-L        1.443      0.094      1.349        14.213               2.3                   1
  Fraction VI 1X-H       3.029      0.094      2.935        6.185               11.5                   1
 Fraction VI X/10-L      0.212      0.094      0.118        12.432              2.3                   10
 Fraction VI X/10-H      0.657      0.094      0.563        11.864              11.5                  10
Fraction VI X/100-L      0.152      0.094      0.058        61.109              2.3                  100
Fraction VI X/100-H      0.333      0.094      0.239        50.362              11.5                 100
Average conc.                  Total protein
Samples          (mg/mL)
                               Volumes (mL)
                                                  (mg)


Fraction I        30.39            65           1974.62

Fraction II       64.16            62           3978.18

Fraction III       5.92            25            147.90

Fraction IV        7.56            21            158.86

Fraction V        34.21            136          4652.61

Fraction VI       33.94            78           2647.45
Fraction VI
                                                     Fraction V
                                                     Fraction V
                                                     Fraction III
                                                     Fraction II
                                                     Fraction I
  250-

         150-

                100-

                       75-


                             50-


                                   37-



                                         25-


                                               15-
PAGE
SDS-
Expected   Obtained
Conclusion
• Our results were not what was expected.
• We were not able to successfully isolate wheat
  germ acid phosphatase.
• This could be accountable to human error
  (bad pipetting, error in making solutions, ).
Acknowledgements

    • Vibha Bansal PhD
    • Edmarie Martinez
  • Vivian Rodriguez Cruz
• Alexandra Rosado Burgos
References
• Stoscheck ,2000. CM. Quantitation of Protein.
  Methods in Enzymology, 50-69.
• Yasuaki Kawarasaki, Hideo Nakano, Tsuneo
  Yamane, 1999. Purification and some
  properties of wheat germ acidphosphatases.
  Elsvier
  [http://www.sciencedirect.com/science/articl
  e/pii/0168945296044779]

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  • 1. Isolation, Purification, and Assay of Wheat Germ Acid Phosphatase Natalia Manzano Wilmarie Morales RISE Program May 10th, 2012
  • 2. Objectives: • To purify and isolate acid phosphatase from wheat germ. • Determine protein concentration using Bicinchoninic Acid protein assay.
  • 3. Introduction • Wheat germ is a very small part of a wheat kernel. • Wheat germ is very high in protein. • It contains around 28% protein and has more protein than can be found in most meat products.
  • 4. Wheat Germ Acid Phosphatase Catalyzes the hydrolysis of phosphate groups from macromolecules and smaller molecules that are stored in the wheat seed. The growing wheat embryo uses the freed phosphate in germination and growth.
  • 5. Materials and Methods Materials 25 g Wheat germ MnCl2, 1.0 M Centrifuge, high Balance H2O, prechilled to 4˚C Sodium acetate speed buffer, 1.0M (pH 5.7) Ice bucket Spectrophotomet Cheesecloth (NH4)2SO4, saturated er, visible (pH 5.5) Magnetic stirrer Microplate Ice, crushed Pasteur Pipets Waterbaths (30˚C and 70˚C) BCA Kit Gloves, disposable BSA standard, 1.0 Weighing trays mg/ml Methods Bicinchoninic Acid protein assay (BCA) SDS PAGE
  • 6. Procedure I: Obtaining Fractions Filter wheat germ * All centrifugation was done at with cheese cloth 2800Xg at 4° for 20min Centrifuge filtrate (70ml) Discard Pellet Fraction I Pellet Add 1.26 ml of MnCl2 1.0M Discard Pellet Add Sodium Acetate Centrifuge Centrifuge Supernatant 62 ml Supernatant 25 ml Fraction II Fraction III
  • 7. Pellet (buffer) Add 33.48 ml of Ammonium Sulfate Centrifuge (Saturated 35%) Supernatant 92 ml Centrifuge Discard Pellet Add 46.92 ml of Supernatant Ammonium Sulfate 21 ml (Saturated 57%) Centrifuge Supernatant 136 ml Fraction IV Pellet Fraction V Suspend in dH2O Centrifuge Fraction Discard Pellet VI
  • 8. Procedure II: • BCA serves the purpose of BCA Assay reacting with complexes between copper ions and peptide bonds to produce a purple end product. • Estimate visually or measure with a standard spectrophotometer or plate reader (562nm).
  • 10.
  • 11. Procedure III: SDS-PAGE • Running Gel: • Stacking Gel: – 1.88 ml dH2O – 2.975 ml dH2O – 1.67 ml separating buffer – 1.25 ml separating buffer – 2.22 ml Acrylamide – 0.662 ml Acrylamide – 50.0 µl 20% SDS – 225.0 µl 20% SDS – 100 µl 10% Glycerol – 25 µl 10% Glycerol – 1.67 µl TEMED – 6.25 µl TEMED – 50 µl APS(100 mg/ml) – 25 µl APS
  • 12. Get sample obtained from previous purifying technique Load Buffer Set up gel, remove comb Load Sample (3:1 sample:buffer) Run Gel Stain with Coomassie and Study Gel Procedure III: SDS
  • 13. Results: Sample Absorbance Blank Abs-Blank Conc. (mg/ml) Vol. of sample added Dilution factor Fraction I 1X-L 2.511 0.094 2.417 25.466 2.3 1 Fraction I 1X-H 3.029 0.094 2.935 6.185 11.5 1 Fraction I X/10-L 0.305 0.094 0.211 22.231 2.3 10 Fraction I X/10-H 1.171 0.094 1.077 22.695 11.5 10 Fraction I X/100-L 0.13 0.094 0.036 37.930 2.3 100 Fraction I X/100-H 0.241 0.094 0.147 30.976 11.5 100 Fraction II 1X-L 3.029 0.094 2.935 30.923 2.3 1 Fraction II 1X-H 3.029 0.094 2.935 6.185 11.5 1 Fraction II X/10-L 0.385 0.094 0.291 30.660 2.3 10 Fraction II X/10-H 1.636 0.094 1.542 32.493 11.5 10 Fraction II X/100-L 0.164 0.094 0.07 73.752 2.3 100 Fraction II X/100-H 0.512 0.094 0.418 88.081 11.5 100 Fraction III 1X-L 0.524 0.094 0.43 4.530 2.3 1 Fraction III 1X-H 2.035 0.094 1.941 4.090 11.5 1 Fraction III X/10-L 0.143 0.094 0.049 5.163 2.3 10 Fraction III X/10-H 0.317 0.094 0.223 4.699 11.5 10 Fraction III X/100-L 0.094 0.094 0 0.000 2.3 100 Fraction III X/100-H 0.138 0.094 0.044 9.272 11.5 100 Fraction IV 1X-L 0.536 0.094 0.442 4.657 2.3 1 Fraction IV 1X-H 1.541 0.094 1.447 3.049 11.5 1 Fraction IV X/10-L 0.149 0.094 0.055 5.795 2.3 10 Fraction IV X/10-H 0.303 0.094 0.209 4.404 11.5 10 Fraction IV X/100-L 0.102 0.094 0.008 8.429 2.3 100 Fraction IV X/100-H 0.163 0.094 0.069 14.540 11.5 100 Fraction V 1X-L 2.373 0.094 2.279 24.012 2.3 1 Fraction V 1X-H 3.029 0.094 2.935 6.185 11.5 1 Fraction V X/10-L 0.179 0.094 0.085 8.956 2.3 10 Fraction V X/10-H 0.673 0.094 0.579 12.201 11.5 10 Fraction V X/100-L 0.151 0.094 0.057 60.055 2.3 100 Fraction V X/100-H 0.358 0.094 0.264 55.630 11.5 100 Fraction VI 1X-L 1.443 0.094 1.349 14.213 2.3 1 Fraction VI 1X-H 3.029 0.094 2.935 6.185 11.5 1 Fraction VI X/10-L 0.212 0.094 0.118 12.432 2.3 10 Fraction VI X/10-H 0.657 0.094 0.563 11.864 11.5 10 Fraction VI X/100-L 0.152 0.094 0.058 61.109 2.3 100 Fraction VI X/100-H 0.333 0.094 0.239 50.362 11.5 100
  • 14. Average conc. Total protein Samples (mg/mL) Volumes (mL) (mg) Fraction I 30.39 65 1974.62 Fraction II 64.16 62 3978.18 Fraction III 5.92 25 147.90 Fraction IV 7.56 21 158.86 Fraction V 34.21 136 4652.61 Fraction VI 33.94 78 2647.45
  • 15.
  • 16.
  • 17. Fraction VI Fraction V Fraction V Fraction III Fraction II Fraction I 250- 150- 100- 75- 50- 37- 25- 15- PAGE SDS-
  • 18. Expected Obtained
  • 19. Conclusion • Our results were not what was expected. • We were not able to successfully isolate wheat germ acid phosphatase. • This could be accountable to human error (bad pipetting, error in making solutions, ).
  • 20. Acknowledgements • Vibha Bansal PhD • Edmarie Martinez • Vivian Rodriguez Cruz • Alexandra Rosado Burgos
  • 21. References • Stoscheck ,2000. CM. Quantitation of Protein. Methods in Enzymology, 50-69. • Yasuaki Kawarasaki, Hideo Nakano, Tsuneo Yamane, 1999. Purification and some properties of wheat germ acidphosphatases. Elsvier [http://www.sciencedirect.com/science/articl e/pii/0168945296044779]