The design of: A Biosensor for glucose detection

in #science7 years ago (edited)

Build your own Biosensor

Development of a Biosensor for glucose detection



screen_printed_elect2.gif

Figure

The actual electrode of model DS 110. The black circle in the middle, called the working electrode. Glucose oxidase and prussian blue will adhered to it via the method of amperometry. We will also use a subclass of amperometry, CV, cyclic voltage, and after designing it, we can apply beverages or fluid samples on the electrode to measure sugar content.


Background

I had some time over the other day, and some glucose oxidase to spare so i decided to design 4 x glucose biosensors for fun, since I had all the needed ingredients. I pulled out an old recipe and design schedule, and made a 1st generation glucose sensor from scratch on a DS 110 carbon diode electrode with an Ag/AgCl counter electrode. The sensor is based on Prussian blue, glucose oxidase and some usage of cyclic voltammetry/amperometry. I chose a cheap and easy to replicate design so you can try it yourself.

generations.PNG

Schematic image showing differences in the generations of biosensors. I used a design from the 1st generation and added an catalytic element, since it covers a lot more chemistry and some engineering as well as is it being the easiest to rerpduce

I will provide the full list of ingredients and a detailed design plan that anyone can follow!
p.s all the images and facts with no references are my own design and I give full rite of usage to everyone in any context.



I measured the sugar content in what I could get my hands on around the laboratory, which was coffee, coffee with sugar, soda, diluted soda and some PBS(who doesn't have that doh)

The first design worked well and here is the data from my trail run. It took me about 4 hours to set up 4 x sensors due to using cyclic voltammetry and the time it requires.

results.PNG




What is biosensors, and what is the glucose sensor used for?



The definition of a biosensor is a sensor for a given analyte, base on biological active system produced in vivo or synthesized to the same structure and function. The biological system creates a unique signal corresponding to the analyte we wish to measure. In the sensor I designed, we measure the amount of hydrogen peroxide that is created by glucose oxidase when it catalyzes the reaction of glucose into gluconic acid. We do this via a catalytic reaction with Prussian blue, containing redox active copper & cyanide ions, which further catalyzes the reaction of hydrogen peroxide and changes the copper & cyanide complex structure and charge. To be precise, It is not a redox mediator, it is a catalytic biosensor. We can trace the amount of copper that changed state exactly via the current we measure over the electrodes, making the sensor pretty precise when manufactured to satisfaction.

diabetes.PNG

Figure

Measuring blood sugar with a glucose sensor, this is an perfect application of our designed sensor, it could even work medicinally with access a known reference sample from the patient

The most common use for the glucose sensor is off course in medicine and especially towards diabetic patients who need to know their level of blood sugar, at home, continuously.

Blood-glucose biosensors usage at home accounts for 85% of the gigantic world market.
https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4862100/

There are many different properties besides electrochemical ones( like the redox mechanism in our design) that can be used to design a biosensor. It can be acoustic , magnetic or optical signals that change due to biochemical events. There are many uses besides the medical industry and the first that comes into mind is the food industry. They need to monitor bacteria and chemical pollutants at a production stage. During the transportation / selling periods, the food is randomly tested for freshens via trace chemicals, all this can be done in a cheap and time saving manner with biosensors.

Fermentation procedures are sensitive to many different changes in chemical composition, and requires some monitoring. Biosensors make it easy to measure e.g oxygen or yeast concentration in a solution or test for unwanted metals / bacteria.

An arduous quandary in food processing industry is of quality and safety, maintenance of food products and processing. Traditional techniques performing chemical experiments and spectroscopy have shortcomings due to human fatigue, are expensive and time consuming. Alternatives for food authentication and monitoring with objective and consistent measurement of food products, in a cost effective manner, are desirable for the food industry. Thus development of biosensors in response to the demand for simple, real-time, selective and inexpensive techniques is seemingly propitious.
https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4862100/

There is always huge demands for new designs of technically supreme biosensors


Principle of our glucose biosensor

There are three common types of generations of biosensors, 1, 2 and third generation biosensors which differ in signal transduction. The different generations of sensors can be seen in the second picture from the top.

An electrochemical glucose biosensor was developed, with a first generation design adding a catalytic element. It consists of three electrodes; a working-, counter- and reference electrode. The potential is measured between a working electrode and a reference electrode. In contrast, current is measured between a working electrode and a counter electrode. The techniques cyclic voltammetry and amperometry was used to activate, functionalize and validate the developed biosensor.

Capture.PNG

The working principle of the biosensor can be seen in Figure 1 and is based on the formation of electroactive molecules. Detection of D-glucose is based on activity of glucose oxidase in the reaction;

reaction1.PNG

Hydrogen peroxide (H2O2) interacts with a ferric ferrocyanide in the redox reaction;

reactioon2.PNG

This reaction produces an anodic current which is measured between a working- and counter electrode.




Ingredients and laboratory setup

Ingridients.PNG

Setup.PNG

Setup from a university I attended

The recipe is common and I used it as a student as well, when taking the course in biosensors, hope you find it usefull.

To send currents between E.g. -0.7 and 0.7 volt, and sweep the range with small increments at a time while measuring the current, you need software and some kind of electrode socket box connected to a potentiostat.

I used PalmSens software PTStrace 5 for windows(they also have electrodes and potentiostat) which will be visible throughout the design, the hardware is shown in the picture above.

PalmSense gear

This is the actual recipe and setup I used so it sure works. If you have any questions about acquiring them or doing dilutions or anything biochemical / laboratory really, leave a comment

The main problems with reproducibility is:


  • pH, sensitive, keep constant and physiological.
  • Temperature, sensitive, must be kept constant.
  • Dynamic range, the largest and smallest possible measurable value, might change somewhat, making it very calibration sensitive.

Step by step design tutorial

This is the actual data from my design, if you try the procedure you should be able to replicate the pattern, no matter the circumstances. I had to use print screen for the captures from PalmSens/PTStrace 5 software, due to the fact that our laboratory computers never connect to the internet or internal net and lacks all software expect the designated one, it came down to this.

1. Chose amperometric detection function from the alternatives in the left screen. The droplet must connect the electrodes in order for this procedure to work, when using a pipette, be sure to cover the entire area!

Step1.PNG


2. Chose cyclic voltammetry and use the specific values i´ve provided unless you got another design going.

step21.PNG

step22.PNG


3. In this step, you can run an extra amperometric response to hydrogen peroxide, but it's fully optional to the basic function of the design.

step31.PNG

step32.PNG


4. This step requires a nice pipette since small volumes must be placed on the working electrode. Place the drops according to the instructions below and let dry.

step4.PNG

  • Preparation of enzyme-nafion electrodes as followed:
  • Place a droplet ~1 µl of the enzyme solution cover all the Prussian blue functionalized electrode surfaces (Reminder: Only place the enzyme/nafion
    solution onto the WORKING ELECTRODE surface). Then, keep the electrodes
    at room temperature for 15 minutes to dry.
  • Place a droplet ~1 µl of the nafion solution onto the electrode surfaces covering the
    all the enzyme layer. Then, keep the electrodes at room temperature for 5 minutes to
    dry

5. The last part is about calibrating the sensor to stock solutions of glucose, which is easily prepared and diluted after your needs.

step5.PNG

curve.PNG

tabel.PNG

If you receive values that are somewhat linear, regress it and put the values in, and we are done!


6.Measure away!

step6.PNG

DS110.PNG

  • Place a drop of your beverage on the electrode as regular.
  • Chose amperometric response with settings like step 3 and 5 then measure the sugar content in soda, coffee or whatever you want to measure. I would also suggest to design 10 of them while you are at it, since there are some troubles with gaining reproducibility in the results when using this method.
  • Diluting the samples can help improving measure quality!
  • Done!

results.PNG

The results are not bad, the lower beverages with low sugar content clearly separate and in the right order.
The more sugary samples is less stable, since the reaction rate can´t be expected to be the same all the time, after the bottom layer is depleted from glucose the signal might get a bit unstable. The medical grade sensors have much more precise delivery mechanisms and thereby much greater sensitivity and takes smaller samples as well.




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This is my first post on a engineering based topic that is not genetic engineering, hope you liked it, I am not sure which is best, to share the full procedure of design or just common facts like everyone else, feel free to comment on this.
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wow, what a response. 143 upvotes. You hit a diabetic nerve

Try the procedure :))

Thanks for your support :) Peace

Quite thorough, high-level stuff.

Now if you design me a complete home blood test kit, that would save me some money!

:P

Well if you had an optimal sample as reference, I think this design could detect a level that is lower, prior to your death :)) but I would´t bet anyone´s life on it, so I ll have to get back to you on that hehe

Growing insuline in E.coli is easier at home I´d say and saves more money perhaps?

Peace

I have never done CV in aqueous solution before... any tips or tricks to get them to look that nice in that medium?

Its sufficiently tricky for me remove oxygen (via purging with nitrogen) from anhydrous organic solvents as it is for CV sometimes.

Hey, I think it is preferred to use aqueous solutions, since it is more flexible, I haven´t tried the other way around, since more specific combinations is needed.

All i know about this topic in organic polar solvents is that we use NBu4PF6, for its inter properties, and I am specialized in proteins sorry ;) So I would rather start at one of these points, then to purge another composition of solvent. Keep pH and temperature exactly stable, so the O2 content is always the same. Use low scan rate ^^

Look at the result screen, It´s not that good! The rest of the Images are cleaned or produced in steps where they always look decent ;)
But if you try a design I got experience from i could point to some problems of reproducability in more detail then the text!

Thanks for reading!

very good post my friend like your post, my resteem and upvote yes

Thanks for checking it out!

Wow, thanks for this post. I'm working on my chemistry bachelor right now, this is a great content!

My pleasure :) Thanks you for checking it out!

Really cool!

Biochemistry in action :)

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