Lab 3.5 Finale



Search



Home



Saved

1

2.0K views



Sign In

Upload

Join

RELATED TITLES

0

Lab 3.5 Finale Uploaded by Alberto Anderson



Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music



Protein Lab Report.docx

1

of 16

 

Biochemistry Lab Report

sds page

 Search document



Experiment 7: Electrophoresis of Protei

Alex Foo (Partner: Matthew Crerar) 5673657 – [email protected]

Bchm 317 – Group 3 TA: Da Duan November 10, 2009

Master your semester with Scribd & The New York Times Special offer for students: Only $4.99/month.

Read Free Foron 30this Days Sign up to vote title



 Not useful Cancel anytime.

Useful

 





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In

Read Free For 30 Days Cancel anytime.

Join





Search



Home



Saved

2.0K views

1



Upload

Sign In

Join

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music




1

of 16

 


sds page

 Search document



Introduction

Electrophoresis Electrophoresis is one of the most versatile tools in analytical biochemistry, a allows separation of proteins and other molecules based on a number of different

properties. However, in order to use electrophoresis effectively in the laboratory, on have a thorough understanding understanding of the mechanism of separation for different electrophoresis electrophoresis methods, and the strengths and limitations of associated with each

method. In this study, Sodium Dodecyl Sulphate Polyacrylamide Gel Electrophoresis

PAGE) is used to separate proteins from samples of purified invertase, invertase, and to determ

the molecular mass of rat Lactate Dehydrogenase (LDH) isozymes. Cellulose Acetat

Electrophoresis Electrophoresis (CAE) is then used to resolve the different LDH isozymes. The prope and limitations of both techniques will be explored during the course of the study.

Material Mater ials s and Methods Metho ds:

All materials and methods used in this laboratory experiment are found in the Quee University 317 lab manual and were used without modification. Master your Bchm semester with [1], Scribd Read Free Foron 30this Days Sign up to vote title & The New York Times  Useful  Not useful Special offer for students: Only $4.99/month.

Cancel anytime.

 





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join





Search



Home



Saved

2.0K views

1



Sign In

Upload

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music

Join




1

of 16

 


sds page

 Search document

Results:



*Note: all tables and figures are sh

the appendix

In this experiment, SDS-PAGE gel electrophoresis was used to determine the

molecular weight of Lactate Dehydrogenase Isozymes (LDH) from rat heart and mus mu

tissue. The molecular weight of carboxypeptidase carboxypeptidase was also measured. Molecular we

measurements were calculated calculated by comparing the distance each of the sample band

migrated to a standard lane loaded with peptides of known molecular weights, weights, as sh

figure 1. The 4 lysosome purification purification fractions from previous experiments were also

the same gel to qualitatively observe the purity of the various fractions. This is done

both observing the size and intensity of the invertase protein band, and the number intensity of other contaminating protein bands on the gel.

The distance migrate and mass of each of the standard proteins was tabulate

table 1, and the data was used to create a standard curve, as shown in figure 2. The

standard curve was used to calculate the molecular weight of the two LDH isozymes

well as the carboxypeptidase. Sample calculations are shown in calculation 1, and t

Master your weights semester with inScribd molecular are tabulated table 1. & The New York Times Special offer for students: Only $4.99/month.





Useful

 

Since the molecular weight of invertase subunits is about 60-63 kDa dependi





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join





Search



Home



Saved

2.0K views

1



Sign In

Upload

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music

Join




1

of 16

 


sds page

 Search document



proteins, and thus its total purity is still low. This matches with previous observation

showing that fraction 2 has the lowest specific activity, but still does not explain the

anomalous result for absolute invertase content. Fractions Fractions 1 and 3 were observed to

lower invertase band intensities, with fraction 3 showing fewer contaminating prote

bands than fractions fractions 2 and 1. This suggests suggests that fraction 3 has both a greater greater abso

invertase content and invertase purity than fraction 1, which correlates to results fro

previous study. A summary of the qualitative observations from the SDS-PAGE of th invertase fractions, and the quantitative results from our previous study are shown table 2.

It was noted that the SDS-PAGE procedure did not produce any significant

separation of the two LDH isozymes. For this reason, it was decided to examine LDH

isozymes using cellulose acetate electrophoresis instead of SDS-PAGE in order to ac

better separation. Samples of LDH from rat heart, kidney and liver tissues were plac

separate cellulose acetate strips. Voltage was then applied lengthwise across the st

separate the different isoforms. The strips were then stained using an “activity stain help visualize the position of the various bands.

Master your semester with Scribd & The New York Times





Useful

 

It was noted that this method gave a much better separation pattern compar Special offer for students: Only $4.99/month.





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join





Search



Home



Saved

2.0K views

1



Sign In

Upload

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music

Join




1

of 16

 


sds page

 Search document



showed two additional bands bracketing position 2, thereby indicating that the hear

sample contains a large number of LDA isozymes, each with a different degree of ch The cellulose electrophoresis electrophoresis results are shown in figure 3, alongside the labels for

position 1, position 2 etc. This separation pattern is much more useful than the sing band at ~60 kDa obtained through SDS-PAGE.






Useful

 





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join





Search



Home



Saved

2.0K views

1



Upload

Sign In

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music

Join




1

of 16

 


sds page

 Search document



Discus Dis cussio sion n: In this laboratory experiment, we initially employed SDS-PAGE as a means protein separation. The basic principle behind gel electrophoresis electrophoresis is that charged molecules such as peptides will migrate through a supporting medium due to an

electrostatic force, brought about by the application of an electric field across the g

speed of migration will depend on the equilibrium equilibrium between the electrostatic force ex

by the electric field, and the opposing frictional and electrophoretic electrophoretic retardation forc

shown in figure 4. SDS is added to the gel in order to give all proteins the same line

unfolded structure and charge to weight ratio. This ensures that they all have the sa

electrostatic force to mass ratio, and that separation occurs based upon the size se

electrophoretic electrophoretic retardation force, thereby allowsing separation based on peptide siz alone. It should be noted that, as a result of the charge/weight ratio homogenizatio

the addition of SDS, it is impossible to determine the native state of the sample pro

based on SDS-PAGE gel results alone. However, it is possible to quantify the molecu

weights of the separated proteins through the use of a standard lane on the gel whi

Master your semester with Scribd  loaded with peptide markers of known molecular weights. By measuring Read Free Foron 30this Days Sign up to vote titlethe distanc  & TheofNew York Times  Useful  Not useful the markers move, it is possible to plot a reproducible, reproducible, linear relationship betwee Special offer for students: Only $4.99/month.

Cancel anytime.

molecular weight, and distance traveled and use it to determine the exact molecula





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join





Search



Home



Saved

2.0K views

1



Upload

Sign In

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music

Join




1

of 16

 


sds page

 Search document



4, which may be due to the accidental cleavage of invertase into smaller peptide ch during the course of the purification experiment. It is known that invertase occurs naturally as a glycoprotein with a mass of 205 kDa [2], of which only 60 kDa make

actual invertase. Thus, it is also possible that the lower molecular mass fragments fragments a

simply due to pieces of the glycoprotein shell of invertase breaking off and physisor Coomassie Blue dye from the staining procedure.

The results also showed that fraction 2 showed two strong bands at about 60

This suggests that fraction 2 contains a high level of invertase, as discussed previou

This contradicts our previous study, which showed that fraction 2 has a lower level o

enzyme activity than both fraction 1 and 3 (see table 2). This result may have been

the fact that the test tubes were mixed up in the previous study, and thus the calcu

protein concentration concentration of fraction 2 may have been wrong. This could have lead to th incorrect dilution of the SDS-PAGE protein sample, and thus the abnormally strong

invertase protein band observed fro fraction two. This would also explain why all the in fraction 2 are more intense than any other fraction examined. Another possible

explanation is that there happens to be a second contaminating protein whose mole weight alsosemester corresponds to 60 kDa. Master your with Scribd  Read Free Foron 30this Days Sign up to vote title  & The NewIf one York Times  Useful  Not useful chooses to disregard fraction fraction 2 for the reasons mentioned earlier, and Special offer for students: Only $4.99/month.

Cancel anytime.

previous report, then the results of the SDS-PAGE separation show that the purity o





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join





Search



Home



Saved

2.0K views

1



Upload

Sign In

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music

Join




1

of 16

 


sds page

 Search document



applied lengthwise across the cellulose acetate support. This support provides a rela

constant frictional retardation force upon the proteins while the electrostatic force p

proteins through the film at a rate dependant on its natural charge: the more negat

protein, the stronger the electrostatic force and the faster it will migrate through th

acetate film. Since separation is not based on size, it is impossible to determine the

the sample proteins based on the cellulose acetate electrophoresis results. It may b

possible to determine qualitatively the native charge of the sample proteins tested.

However, it is doubtful whether the relationship between charge and distance migra

linear or reproducible. Since CAE relies on the proteins’ native charge to function, th

of SDS should be avoided, as it will eliminate the difference in the proteins’ native c and thus make separation impossible. impossible.

In order to visualize the results of the electrophoresis separations, separations, one must h method for staining the protein bands on the gels. In the SDS-PAGE study, we were to identify all the protein bands, and thus the Coomassie blue dye was chosen for

ability to indiscriminately dye all proteins and peptides. In the cellulose acetate stud

however, we were only concerned with the LDH peptides, and did not want any inte

bands fromsemester contaminant proteins. Thus, we used an “activity stain” to produce Master your with Scribd  colo Read Free Foron 30this Days Sign up to vote title  where LDH was present. & Thebands Newonly York Times  Useful  Not useful Special offer for students: Only $4.99/month.

Cancel anytime.

The CAE studies show the presence of varying amounts of isozymes in the dif





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join





Search



Home



Saved

2.0K views

1



Upload

Sign In

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music

Join




1

of 16

 


sds page

 Search document



bands observed by both ourselves and [6]. In contract to this, the heart tissue cells

produce almost equal amounts of both subunits, which leads to the presence of 5 d isozymes [6]. However, the prevalence of one of these isozymes is about 1% [6],

makes it almost impossible to detect using our CAE method, and thus only 4 isozym

observed. The kidney tissue was observed observed to produce only one band, band, which sugges

rat kidney tissue cells produce only one type of subunit, and thus only one isozyme

possible. However, this was not found to be the case in [6]. This discrepancy could b

to the fact that cells from different parts of the kidney could express different prote

and thus lead to variability between samples of the same tissue. For example, exerc

and metabolic activity may affect the expression of various isozymes [7], and thus l

variability in CAE results. results. A full comparison comparison between our results results and that of from lit is shown in table 3.

Sources Sour ces of o f Error Er ror : As mentioned previously in the discussion, sources of error could have been

propagated up from the previous studies, and have lead to incorrect dilutions of our

invertase fractions, particularly particularly for fraction 2. Other sources of error include the fact

Master your semester with Scribd  the expressed proteome for a cell varies with environmental conditio ns, Read Free Foron 30this Days Sign up to conditions, vote titleand even th  & TheofNew York Times  Useful  Not useful the tissue from which it was extracted. As discussed in the discussion, this could Special offer for students: Only $4.99/month.

Cancel anytime.

lead to discrepancies between the number of LDH isozymes identified in our study,





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join





Search



Home



Saved

2.0K views

1



Sign In

Upload

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music

Join




1

of 16

 


sds page

 Search document



experiments. We were also able to determine the molecular weight of two different LDH isozymes. Although these values matched those of literature, they were too

together to allow proper resolution via SDS-PAGE. As a result, CAE was employed on

samples of LDH from 3 different tissues. This method was able to differentiate betw

the different isozymes, and the results roughly corresponded to literature research,

some exceptions. In using these two techniques, techniques, the principles, principles, limitations limitations and pos applications of various types of electrophoresis electrophoresis were revealed and discussed.






Useful

 





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join





Search



Home



Saved

2.0K views

1



Upload

Sign In

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music

Join




1

of 16

 


sds page

 Search document



Sources Cited

1. Prosser, David E., and Vinay K. Singh. (2009) BCHM317 Laboratory Manual 2009Queens University, Kingston. pp. 35-37

2. Moreno, S., Sanchez, Y., and Luis Rodriguez. (1990) Purification Purification and Characteriza

the Invertase from Schizosaccharomyces pombe – a Comparative Analysis wi Invertase from Saccaromyces Saccaromyces cerevisiae. cerevisiae. Biochem. J. 267. pp. 697-702

3. Trimble, R.B., and Frank Maley. (1997) Subunit Structure of External Invertase fro

Saccaromyces cerevisiae. The Journal of Biological Chemistry 252(12). pp 440 4412.

4. Neumann, N. P., and J. O. Lampen. (1967) Purification Purification of Yeast Invertase. Biochem 6(2). pp 468-475

5. Goodwin, A.B., Schneider, R.E., and William E. Fry. (1995) Use of Cellulose-Acetat

Electrophoresis Electrophoresis for Rapid Identification of Allozyme Genotypes of Phytophtho infestans. infestans. Plant Disease 79(11). pp. 1181-1185.

Master your semester with Scribd  Read Free Foron 30this Days Sign up to vote title  Nadal-Ginard, Bernardo. (1978) Regulation of Lactate Dehydrogenase & The6.New York Times  Useful  Not useful Levels in th Special offer for students: Only $4.99/month.

Cancel anytime.

Mouse. The journal of Biological Chemistry. 253(1). pp. 170-177





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join





Search



Home



Saved

2.0K views

1



Upload

Sign In

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music

Join




1

of 16

 


sds page

 Search document



Appendix:

Figure 1: Stained SDS-PAGE gel after electrophoresis of rat heart and muscl

isozymes, carboxypeptidase, carboxypeptidase, and the various invertase fractions collected fro

previous experiments. Lane 4 is the standard lane, with the molecular weight

labeled. Master your semester with Scribd  Read Free Foron 30this Days Sign up to vote title  & TheFigure New2:York Times Useful  Not useful  Standard curve for migration distance of the various bands vs the log of t Special offer for students: Only $4.99/month.

Cancel anytime.

molecular weight. The linear regression for the linear section of the graph is shown.





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join





Search



Home



Saved

2.0K views

1



Sign In

Upload

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Magazines



News



Documents



Sheet Music




1

Download



Join

 

of 16

Markers

LDH(M4) LDH(H4) Carboxypepti dase Invertase


sds page

 Search document

2 50 1 50 1 00 75 50 37 25 20 15 10 35 35

0.2 0.3 0.4 0.6 1.1 1.5 2.1 2.7 3.2 3.9 1.7 1.7

31* 56

1.9* 0.9



Calculation 1: Determining the molecular weight of Carboxypeptidase through its migration distance as observed during SDS-PAGE analysis. logMW=-0.256X+1.983 logMW=-0.256X+1.98 3

X = Distance migrated, X = 1.9cm

logMW=-0.2561.9+1.983 logMW=1.4966

Master your semester with Scribd MW=31.376 & The New York Times MW=31kDa Special offer for students: Only $4.99/month.





Useful

 





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join





Search



Home



Saved

2.0K views

1



Sign In

Upload

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music

Join




1

of 16

 


sds page

 Search document



Figure 3.1, 3.2: Image of the developed CAE films showing the separation o different rat tissue LDH isozymes.






Useful

 





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join





Search



Home



Saved

2.0K views

1



Sign In

Upload

Join

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music




1

of 16

 


sds page



 Search document

Table 2: Tabulated qualitative values for invertase sample purity as determined fro

figure 1, compared to the invertase sample purity as determined in our previous stu

denoted the most pure, and 4 denotes the least pure, as determined by the SDS-PA analysis. Fracti Specific Activity, U/mg(From Purity (from SDS-PAGE, on lab 6) Experiment 7) 1 2865 2 216.9 3 3655 4 5039


4 2 3 1





Useful

 





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join





Search



Home



Saved

2.0K views

1



Sign In

Upload

RELATED TITLES

0




Top Charts



Books



Audiobooks









Save

Embed

Share

Print

Download



Magazines



News



Documents



Sheet Music

Join




1

of 16

 


sds page

 Search document



Table 3: Comparison Comparison of the LDH isozymes present in the various rat tissues as determined by our experiment and literature results [6]. Tissue

Experimental va values

Heart Kidne y Liver

4 iis sozymes ob observed 1 isozyme observed 2 isozymes observed

Literature va values [6 [6] 5 isozymes present, One of these occurs in trace amounts only 5 isozymes present, all occur in significant amounts 2 isozymes observed






Useful

 





Home



Saved



Top Charts



Books



Audiobooks



Magazines



News



Documents



Sheet Music




Upload

Sign In


Join



Lab 3.5 Finale

Recommend Documents