BME100 s2014:T Group13 L5: Difference between revisions

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The Fluorimeter allows for the quantitative evaluation of samples that underwent a Polymerase Chain Reaction (PCR). It is made up of an interior black box, or table, plastic trays, a slide port, a blue excitation light, a camera phone cradle, a Samsung galaxy s4 camera phone, and an exterior black box that covers all other components.
The Fluorimeter allows for the quantitative evaluation of samples that underwent a Polymerase Chain Reaction (PCR). It is made up of an interior black box, or table, plastic trays, a slide port, a blue excitation light, a camera phone cradle, a Samsung galaxy s4 camera phone, and an exterior black box that covers all other components.


The first component, the interior black box, basically acts as both a table for the slide port and a house for the blue excitation light. The plastic trays sit under this interior box and allows researchers to correctly line up the slide samples and the camera they are using. The slide port is the narrow canal in which the sample slides sit. This port allows for the all samples to be easily interchanged. The blue excitation light is a light that is shone through the samples. The next component is the camera phone cradle and the camera phone (Samsung Galaxy s4). The camera phone is used to take high quality pictures of the samples so that they can then be transferred to a computer. The cradle simply holds the camera in one place. The last component is the exterior black box. This box covers all other components and keeps all unwanted light away from the experiment.  
The first component, the interior black box, acts as both a table for the slide port and a house for the blue excitation light. The plastic trays sit under this interior box and allows researchers to correctly line up the slide samples and the camera they are using. The slide port is the narrow canal in which the sample slides sit. This port allows for the all samples to be easily interchanged. The blue excitation light is a light that is shone through the samples. The next component is the camera phone cradle and the camera phone (Samsung Galaxy s4). The camera phone is used to take high quality pictures of the samples so that they can then be transferred to a computer. The cradle simply holds the camera in one place. The last component is the exterior black box. This box covers all other components and keeps all unwanted light away from the experiment.  
   
   


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** Saturation: N/A
** Saturation: N/A
** Contrast: N/A
** Contrast: N/A
 
<br>
'''Calibration'''<br>
'''Calibration'''<br>
The camera was placed on the camera phone cradle. Plastic slides were placed under the interior black box (on which the sample slides sit), in order to line up the camera on the phone and the sample. The camera was placed 11.0 cm away from the drop in every sample in order to reduce error.  
The camera was placed on the camera phone cradle. Plastic slides were placed under the interior black box (on which the sample slides sit), in order to line up the camera on the phone and the sample. The camera was placed 11.0 cm away from the drop in every sample in order to reduce error.  
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[[Image:Setupcalibration.PNG|400px]]
[[Image:Setupcalibration.PNG|400px]]
* Distance between the smart phone cradle and drop = 11.0 cm
* Distance between the smart phone cradle and drop = 11.0 cm
''[Instructions: See worksheet page 6.]''




'''Solutions Used for Calibration''' ''[Instructions: See worksheet page 6.]''
'''Solutions Used for Calibration'''  
{| {{table}} width=700
{|
| align="center" style="background:#f0f0f0;"|'''Initial<br>Concentration of<br>2X Calf Thymus<br>DNA Solution<br>(μg/mL)'''
| align="center" style="background:#f0f0f0;"|'''Final<br>Concentration of<br>2X Calf Thymus<br>DNA Solution<br>(μg/mL)'''
| align="center" style="background:#f0f0f0;"|'''RawIntDen<br>Values'''
|-
|-
| row 1 cell 1 || row 1 cell 2 || row 1 cell 3 || row 1 cell 4
| 5||2.5||13925853
|-
|-
| row 2 cell 1 || row 2 cell 2 || row 2 cell 3 || row 2 cell 4
| 1||0.5||4240583
|-
|-
| row 3 cell 1 || row 3 cell 2 || row 3 cell 3 || row 3 cell 4
| 0.25||0.125||2746585
|}
|}
''[Add more rows as needed]''
'''Placing Samples onto the Fluorimeter'''
The first step to introducing the samples onto the Fluorimeter was having the Cyber Green solution, the varying samples of DNA samples, two micropipettes each set at 80 micro liters, a plethora of pipette tips, and having the slide positioned in the correct place.
The second step was to put 80 micro liters of the Cyber Green in the center of the slide so that the Blue Excitation Light would shine through it, using one micropipette and discarding the tip afterwards into a cup.
The third step was putting 80 micro liters of a determined sample onto the 80 micro liters of Cyber Green solution with the other micropipette, discarding the tip afterwards into the same cup.


The fourth step was to take a photo using the Samsung Galaxy S4, while having the exterior black box fully closed.
The fifth step was to use one of the micropipettes to take off the combined Cyber Green, DNA solution from the slide, discarding the solution into a specified cup.
The sixth and final step was to move the slide so that contamination wouldn’t happen.


'''Placing Samples onto the Fluorimeter''' <br>
1. Place slide onto the slide port <br>
2. Place 80 micro liters of the SBYR green dye onto the slide in the correct spot<br>
3. Place 80 micro liters of the sample directly on top of the SBYR green dye<br>
4. Shine the blue excitation light through the sample<br>
5. Place the exterior black box, or the light box, over the other components<br>
6. Take 3 pictures of each sample using the smart phone<br>
7. Pipet the sample and dye off the slide and discard<br>
8. Move the sample slide down so that the next area of the slide lines up with the camera<br>
9. Using a new pipet tip for each sample, repeat steps 2-8 for each sample. <br>


<br>
<br>
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'''Image J Values for All Samples'''  
'''Image J Values for All Samples'''  
 
{|
''[Instructions: See worksheet page 8. '''To save time on typing a new Wiki table from scratch''', use THIS TOOL to auto-generate a Wiki table: [http://excel2wiki.net/wikipedia.php Excel-to-Wiki Converter]. Copy the headers and values from the Excel spreadsheet you made, paste them into the form field, click submit, copy the Wiki code that the tool generated, and replace TABLE GOES HERE (below) with your auto-generated code.]''
| align="center" style="background:#f0f0f0;"|'''PCR<br>Product<br>TUBE LABEL'''
 
| align="center" style="background:#f0f0f0;" colspan="3" |'''INTDENS VALUES BASED ON 3 SEPARATE<br>DROP MEASUREMENTS'''
 
|-
TABLE GOES HERE
| nD||561661||5531880||1474683
|-
| pm1||5112480||2339670||2692118
|-
| pm2||1031159||1539857||2605182
|-
| pm3||706705||2215671||8522889
|-
| dD||1999426||4045231||1905225
|-
| pf1||3353278||3749157||3023811
|-
| pf2||2921301||2075295||2876218
|-
| pf3||3112790||4757363||4133227
|}




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'''PCR Results Summary'''
'''PCR Results Summary'''


Instructor's summary: You completed 8 PCR reactions in a previous lab. You used the SYBR Green I staining and imaging technique to measure the amount of amplified DNA in each PCR reaction. You used a standard curve (based on known concnetration of claf thymus DNA) to convert INTDEN values into DNA concentration. Your positive control and negative control samples are used to determine the '''threshold''' values for determining whether an unknown (patient) sample is truly positive or negative.
Instructor's summary: You completed 8 PCR reactions in a previous lab. You used the SYBR Green I staining and imaging technique to measure the amount of amplified DNA in each PCR reaction. You used a standard curve (based on known concentration of calf thymus DNA) to convert INTDEN values into DNA concentration. Your positive control and negative control samples are used to determine the '''threshold''' values for determining whether an unknown (patient) sample is truly positive or negative.
*Positive control PCR result: 1.58851350207904 μg/mL (?)
*Positive control PCR result: 13.94 μg/mL
*Negative control PCR result: 1.26725982132786 μg/mL (?)
*Negative control PCR result: 3.07 μg/mL




Write-in each patient ID and give both a qualitative (what the images looked like) and a quantitative description (μg/mL) of what you observed
Write-in each patient ID and give both a qualitative (what the images looked like) and a quantitative description (μg/mL) of what you observed
*Patient _____ :  
*Patient 41731 F: All of this patient's samples illuminated to various degrees. The concentration values for this patient ranged from 3.21 to 5.04 μg/mL.
*Patient _____ :  
*Patient 78042 M: None of this patient's samples illuminated. The concentration values for this patient ranged from 2.01 to 4.80 μg/mL.


Compare each patient's results to the positive control value and the negative control value. Draw a final conclusion for each patient (positive or negative) and explain why you made that conclusion.
Compare each patient's results to the positive control value and the negative control value. Draw a final conclusion for each patient (positive or negative) and explain why you made that conclusion.
*Patient _____ :  
*Patient 41731 F: This patient's results were much closer to the negative control value, which indicates a negative result.
*Patient _____ :  
*Patient 78042 M: This patient's results were much closer to the negative control value, which indicates a negative result.




Latest revision as of 11:42, 17 April 2014

BME 100 Spring 2014 Home
People
Lab Write-Up 1 | Lab Write-Up 2 | Lab Write-Up 3
Lab Write-Up 4 | Lab Write-Up 5 | Lab Write-Up 6
Course Logistics For Instructors
Photos
Wiki Editing Help


OUR TEAM

Name: Mikaela Hall
Name: Sarah McBryan
Name: Avery Witting
Name: Dan Saunders


LAB 5 WRITE-UP

Background Information

SYBR Green Dye
SYBR Green dye was added to each of the samples from the PCR on the sample slides. A drop of each sample was placed onto a drop of this green dye each time the Fluorimeter was used. These drops of dyes react with different molecules of DNA. In the samples which had no DNA, these reactions didn’t take place. The reaction between the DNA and the green dye cause the blue excitation light to be absorbed and a green light to be emitted. Thus the samples with DNA shone green and the samples without DNA simply shone the original blue from the excitation light. The exterior black box, or light box, is used in order keep all other light from interfering with the images being captured.


Single-Drop Fluorimeter
The Fluorimeter allows for the quantitative evaluation of samples that underwent a Polymerase Chain Reaction (PCR). It is made up of an interior black box, or table, plastic trays, a slide port, a blue excitation light, a camera phone cradle, a Samsung galaxy s4 camera phone, and an exterior black box that covers all other components.

The first component, the interior black box, acts as both a table for the slide port and a house for the blue excitation light. The plastic trays sit under this interior box and allows researchers to correctly line up the slide samples and the camera they are using. The slide port is the narrow canal in which the sample slides sit. This port allows for the all samples to be easily interchanged. The blue excitation light is a light that is shone through the samples. The next component is the camera phone cradle and the camera phone (Samsung Galaxy s4). The camera phone is used to take high quality pictures of the samples so that they can then be transferred to a computer. The cradle simply holds the camera in one place. The last component is the exterior black box. This box covers all other components and keeps all unwanted light away from the experiment.



How the Fluorescence Technique Works
SYBR Green I is a DNA binding dye. In our lab experiment, it was added to samples after the DNA was amplified in a polymerase chain reaction (PCR). These samples were then placed in a Single-Drop Fluorimeter, where a laser/light was shown through the sample towards a camera. The dye attaches to the double stranded DNA and absorbs blue light while reflecting green light. In other words, it glows green when double stranded DNA is present, but it does not glow in water or in the presence of single stranded DNA. After doing a single drop fluorescence test, the amount of SYBR green dye, or green light emitted, was quantitatively graphed using a program called ImageJ. From these graphs, the concentration of DNA was calculated.



Procedure

Smart Phone Camera Settings

  • Type of Smartphone: Samsung Galaxy S4
    • Flash: Off
    • ISO setting: 800
    • White Balance: Auto
    • Exposure: +2
    • Saturation: N/A
    • Contrast: N/A


Calibration
The camera was placed on the camera phone cradle. Plastic slides were placed under the interior black box (on which the sample slides sit), in order to line up the camera on the phone and the sample. The camera was placed 11.0 cm away from the drop in every sample in order to reduce error.

  • Distance between the smart phone cradle and drop = 11.0 cm


Solutions Used for Calibration

Initial
Concentration of
2X Calf Thymus
DNA Solution
(μg/mL) 		Final
Concentration of
2X Calf Thymus
DNA Solution
(μg/mL) 		RawIntDen
Values
5 2.5 13925853
1 0.5 4240583
0.25 0.125 2746585


Placing Samples onto the Fluorimeter
1. Place slide onto the slide port
2. Place 80 micro liters of the SBYR green dye onto the slide in the correct spot
3. Place 80 micro liters of the sample directly on top of the SBYR green dye
4. Shine the blue excitation light through the sample
5. Place the exterior black box, or the light box, over the other components
6. Take 3 pictures of each sample using the smart phone
7. Pipet the sample and dye off the slide and discard
8. Move the sample slide down so that the next area of the slide lines up with the camera
9. Using a new pipet tip for each sample, repeat steps 2-8 for each sample.


Data Analysis

Representative Images of Samples

A sample with no DNA.
A sample with DNA.


Image J Values for All Samples

PCR
Product
TUBE LABEL 		INTDENS VALUES BASED ON 3 SEPARATE
DROP MEASUREMENTS
nD 561661 5531880 1474683
pm1 5112480 2339670 2692118
pm2 1031159 1539857 2605182
pm3 706705 2215671 8522889
dD 1999426 4045231 1905225
pf1 3353278 3749157 3023811
pf2 2921301 2075295 2876218
pf3 3112790 4757363 4133227


Fitting a Straight Line
[Instructions: Place an IMAGE of your Excel plot with a line of best fit here. See worksheet page 9]


PCR Results Summary

Instructor's summary: You completed 8 PCR reactions in a previous lab. You used the SYBR Green I staining and imaging technique to measure the amount of amplified DNA in each PCR reaction. You used a standard curve (based on known concentration of calf thymus DNA) to convert INTDEN values into DNA concentration. Your positive control and negative control samples are used to determine the threshold values for determining whether an unknown (patient) sample is truly positive or negative.

  • Positive control PCR result: 13.94 μg/mL
  • Negative control PCR result: 3.07 μg/mL


Write-in each patient ID and give both a qualitative (what the images looked like) and a quantitative description (μg/mL) of what you observed

  • Patient 41731 F: All of this patient's samples illuminated to various degrees. The concentration values for this patient ranged from 3.21 to 5.04 μg/mL.
  • Patient 78042 M: None of this patient's samples illuminated. The concentration values for this patient ranged from 2.01 to 4.80 μg/mL.

Compare each patient's results to the positive control value and the negative control value. Draw a final conclusion for each patient (positive or negative) and explain why you made that conclusion.

  • Patient 41731 F: This patient's results were much closer to the negative control value, which indicates a negative result.
  • Patient 78042 M: This patient's results were much closer to the negative control value, which indicates a negative result.




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