# 20.109(S13):Assess protein function (Day8)

### From OpenWetWare

(→Protocols) |
|||

Line 1: | Line 1: | ||

- | |||

{{Template:20.109(S13)}} | {{Template:20.109(S13)}} | ||

Line 81: | Line 80: | ||

#If your mutant proteins are not well-described by any of the models so far, what kind of model(s) (qualitatively speaking) do you think might be useful? | #If your mutant proteins are not well-described by any of the models so far, what kind of model(s) (qualitatively speaking) do you think might be useful? | ||

#*Optional: If your data might be well-described by a model with two KD's (or if you are interesting in exploring some sample data that is), download and run [[Media:Fit_TwoKD.m | Fit_TwoKD]] and [[Media:Fit_TwoKD_Func.m | Fit_TwoKD_Func]]. | #*Optional: If your data might be well-described by a model with two KD's (or if you are interesting in exploring some sample data that is), download and run [[Media:Fit_TwoKD.m | Fit_TwoKD]] and [[Media:Fit_TwoKD_Func.m | Fit_TwoKD_Func]]. | ||

+ | |||

+ | ==For next time== | ||

+ | |||

+ | #Results outline | ||

+ | #Extra credit, OR REQUIRED THIS YEAR?: Prepare a figure and caption for your SDS-PAGE, along with a paragraph of text for the associated results section. Look up the expected molecular weight using the IPC sequence document and [http://www.bioinformatics.org/sms/prot_mw.html this] or a similar website. Be sure to add ~ 3 KDa for the size of the N-terminus of pRSET (His tag, etc). If you see two strong bands, what do you think the second one is? |

## Revision as of 12:46, 30 March 2013

## Contents |

## Introduction

This is it, folks! Moment of truth. Time to find out how the proteins that you worked so hard to make and purify really behave. you will analyze the raw data obtained today. Although you should be able to produce reasonable titration curves by following the example of Nagai, the introduction/review of binding constants below may help contextualize your analysis.

Let’s start by considering the simple case of a receptor-ligand pair that are exclusive to each other, and in which the receptor is monovalent. The ligand (L) and receptor (R) form a complex (C), which reaction can be written

At equilibrium, the rates of the forward reaction (rate constant = *k*_{f}) and reverse reaction (rate constant = *k*_{r}) must be equivalent. Solving this equivalence yields an equilibrium dissociation constant *K*_{D}, which may be defined either as *k*_{r} / *k*_{f}, or as [*R*][*L*] / [*C*], where brackets indicate the molar concentration of a species. Meanwhile, the fraction of receptors that are bound to ligand at equilibrium, often called *y* or θ, is *C* / *R*_{TOT}, where *R*_{TOT} indicates total (both bound and unbound) receptors. Note that the position of the equilibrium (i.e., *y*) depends on the starting concentrations of the reactants; however, *K*_{D} is always the same value. The total number of receptors *R*_{TOT}= *[C]* (ligand-bound receptors) + *[R]* (unbound receptors). Thus,

where the right-hand equation was derived by algebraic substitution. If the ligand concentration is in excess of that of the receptor, *[L]* may be approximated as a constant, *L*, for any given equilibrium. Let’s explore the implications of this result:

- What happens when
*L*<<*K*_{D}?

- →Then
*y*~*L*/*K*_{D}, and the binding fraction increases in a first-order fashion, directly proportional to*L*.

- →Then

- What happens when
*L*>>*K*_{D}?

- →In this case
*y*~1, so the binding fraction becomes approximately constant, and the receptors are saturated.

- →In this case

- What happens when
*L*=*K*_{D}?

- →Then
*y*= 0.5, and the fraction of receptors that are bound to ligand is 50%. This is why you can read*K*_{D}directly off of the plots in Nagai’s paper (compare Figure 3 and Table 1). When y = 0.5, the concentration of free calcium (our*[L]*) is equal to*K*_{D}.**This is a great rule of thumb to know.**

- →Then

The figures at below demonstrate how to read *K*_{D} from binding curves. You will find semilog plots right particularly useful today, but the linear plot (left) can be a helpful visualization as well. Keep in mind that every *L* value is associated with a particular equilbrium value of *y*, while the curve as a whole gives information on the global equilibrium constant *K*_{D}.

Of course, inverse pericam has multiple binding sites, and thus IPC-calcium binding is actually more complicated than in the example above. The *K*_{D} reported by Nagai is called an ‘apparent *K*_{D}’ because it reflects the overall avidity of multiple calcium binding sites, not their individual affinities for calcium. Normally, calmodulin has a low affinity (N-terminus) and a high affinity (C-terminus) pair of calcium binding sites. However, the E104Q mutant, which is the version of CaM used in inverse pericam, displays low-affinity binding at both termini. Moreover, the Hill coefficient, which quantifies cooperativity of binding in the case of multiple sites, is reported to be 1.0 for inverse pericam. This indicates that inverse pericam behaves as if it were binding only a single calcium ion per molecule. Thus, wild-type IPC is well-described by a single apparent *K*_{D}.

When you write your research article, be sure to consider how changes in both binding affinity and cooperativity can affect the practical utility of a sensor.

## Protocols

Begin by applying the practice analysis from Day 3, Part 5 of this module to your real data. Recall that here you plot titration curves in Excel and make a first crude estimate of K_{D} values. Next, you will use MATLAB to get improved estimates of K_{D}s and also assess cooperativity. **The MATLAB code is now up to date.**

#### Preparation

- Download these three files: S12_Fit_Main, Fit_SingleKD, and Fit_KDn. If using a computer in 16-336, the files will be available in the
*Downloads*folder under your username. Move them to the username/Documents/MATLAB folder on your PC. - Double-click on the MATLAB icon to start up this software.
- The main window that opens is called the command window: here is where you run programs (or directly input commands) and view outputs. You can also see and access the command history, workspace, and current directory windows, but you likely won’t need to today.
- In the command window, type
*more on*; this command allows you to scroll through multi-page output (using the spacebar), such as help files. - In addition to the command area, MATLAB comes with an editor. Click
*File*→*Open*and select the program**S12_Fit_Main**. It has the .m extension and thus is executable by MATLAB. Read the introductory comments (the beginning of a comment is indicated by a % sign), and then input your fluorescence data. - Read through the program, and as you encounter unfamiliar terms, return to the workspace and type
*help functioname*. Feel free to ask questions of the teaching faculty as well.- You might read about such built-in functions as
*logspace*and*nlinfit*. - You will also want to open and read
**Fit_SingleKD**– a user-defined function called by**S12_Fit_Main**– in the MATLAB editor. - If you type
*help function*you will learn the syntax for a function header. - Note that a dot preceeding an operator (such as A ./ B or A .* B) is a way of telling MATLAB to perform element-by-element rather than matrix algebra.
- Also note that when a line of code is
*not*followed by a semi-colon, the value(s) resulting from the operation will be displayed in the command window.

- You might read about such built-in functions as

#### Analysis

- Once you more-or-less follow Part 1 of the program, type
**S12_Fit_Main**in the workspace, hit return to run the program, and consider the following questions:- Why must the fluorescence data be transformed (from
*S*to*Y*) prior to use in the model? - What
*K*_{D}values are output in the command window, and how do they compare to the values you estimated from your Excel plots? - Figure 1 should display your wild type and mutant data points and model curves. How do they look in comparison to the curves you plotted in Excel?
- Figure 2 should display the residuals (difference between data and model) for your three proteins. If the absolute values are low, this indicates good agreement between the model and the data numerically. Whether or not this is the case, another thing to look for is whether the residuals are evenly and randomly distributed about the zero-line. If there is a pattern to the errors, likely there is a systematic difference between the data and the model, and thus the model does not reflect the actual binding process well. What are the residuals like for each of your modeled proteins?

- Why must the fluorescence data be transformed (from
- Now move on to Part 2 of the
**S12_Fit_Main**program. Part 2 also fits the data to a model with a single, ‘apparent’ value of*K*_{D}, but it allows for multiple binding sites and tests for cooperativity among them. The parameter used to measure cooperativity is called the Hill coefficient. A Hill coefficient of 1 indicates independent binding sites, while greater or lesser values reflect positive or negative cooperativity, respectively. Let the following questions guide you as you proceed:- Visually, which model appears to fit your wild-type data better (Fig. 3 vs. Fig. 1)? Your mutant data?
- Do the respective residuals support your qualitative assessment (Fig. 4 vs. Fig. 2)?
- Numerically, how do the values of
*K*_{D}compare for the two models? How does the value of*n*compare to the implicitly assumed value in Part 1? - Do you see changes in binding affinity and/or cooperativity between the wild-type, E67K/T79P/M124S, and X#Z samples? Do they match your
*a priori*predictions? **Don't forget to save any figures you want to use in your report!**If the legends are covering up your data, you can simply move them over with your mouse.

- Finally, you can skim Part 3 of the
**S12_Fit_Main**program. Don’t worry too much about the coding details, but do read through the comments.- Look at Part 1 of Figure 5: are the binding curves asymptotic, sigmoidal, or other? What does this shape indicate? You can use the zoom button to get a closer look at part of the plot, or the
*axis*command present in the code. (Don't worry too much about this question if it is unclear.) - Now look in the command window. What values of
*K*_{D}and Hill coefficient (*n*) do you get for your three proteins? How do the*K*_{D}’s from Part 3 compare to the ones from Parts 1 and 2? Don’t be discouraged if your wild-type values do not exactly match Nagai’s work, or if there is variation between Parts 1, 2, and 3. - Comparing the model and data points by eye (Part 2 of Figure 5), do you think it is a good model for any of your proteins? If so, which ones? What experimental limitations might prevent Hill analysis from working well, especially for some mutants?
- Why should only the transition region be analyzed in a Hill plot?
- What is the relationship between slope and
*K*_{D}and/or*n*, and intercept and*K*_{D}and/or*n*?

- Look at Part 1 of Figure 5: are the binding curves asymptotic, sigmoidal, or other? What does this shape indicate? You can use the zoom button to get a closer look at part of the plot, or the
- If your mutant proteins are not well-described by any of the models so far, what kind of model(s) (qualitatively speaking) do you think might be useful?
- Optional: If your data might be well-described by a model with two KD's (or if you are interesting in exploring some sample data that is), download and run Fit_TwoKD and Fit_TwoKD_Func.

## For next time

- Results outline
- Extra credit, OR REQUIRED THIS YEAR?: Prepare a figure and caption for your SDS-PAGE, along with a paragraph of text for the associated results section. Look up the expected molecular weight using the IPC sequence document and this or a similar website. Be sure to add ~ 3 KDa for the size of the N-terminus of pRSET (His tag, etc). If you see two strong bands, what do you think the second one is?