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'''Absolute Molar Mass''' is a process used to determine the characteristics of [[molecule]]s.
 
__TOC__
 
== History ==
The first [[absolute measurements]] of molecular weights (i.e. made without reference to standards) were based on [[fundamental physical characteristic]]s and their relation to the molar mass. The most useful of these were [[Osmometry|membrane osmometry]] and [[sedimentation]].
 
Another absolute instrumental approach was also possible with the development of [[light scattering]] theory by [[Einstein]], [[Chandrasekhara Venkata Raman|Raman]], [[Peter Debye|Debye]], [[Bruno H. Zimm|Zimm]], and others. The problem with measurements made using membrane osmometry and sedimentation was that they only characterized the bulk properties of the [[polymer]] sample. Moreover, the measurements were excessively time consuming and prone to [[operator error]]. In order to gain information about a [[polydisperse]] mixture of molar masses, a method for separating the different sizes was developed. This was achieved by the advent of [[size exclusion chromatography]] (SEC).  SEC is based on the fact that the pores in the packing material of [[chromatography|chromatography columns]] could be made small enough for molecules to become temporarily lodged in their interstitial spaces. As the sample makes its way through a column the smaller molecules spend more time traveling in these void spaces than the larger ones, which have fewer places to "wander". The result is that a sample is separated according to its [[hydrodynamic volume]] <math>V_h</math>. As a consequence, the big molecules come out first, and then the small ones follow in the elutent. By choosing a suitable column packing material it is possible to define the resolution of the system.  Columns can also be combined in series to increase resolution or the range of sizes studied.
 
The next step is to convert the time at which the samples eluted into a measurement of molar mass.  This is possible because if the molar mass of a standard were known, the time at which this standard eluted should be equal to a specific molar mass. Using multiple standards, a [[calibration curve]] of time versus molar mass can be developed. This is significant for polymer analysis because a single polymer could be shown to have many different components, and the complexity and distribution of which would also affect the physical properties.  However this technique has shortcomings. For example, unknown samples are always measured in relation to known standards, and these standards may or may not have similarities to the sample of interest. The measurements made by SEC are then mathematically converted into data similar to that found by the existing techniques.
 
The problem was that the system was calibrated according to the Vh characteristics of polymer standards that are not directly related to the molar mass. If the relationship between the molar mass and Vh of the standard is not the same as that of the unknown sample, then the calibration is invalid. Thus, to be accurate, the calibration must use the same polymer, of the same conformation, in the same eluent and have the same interaction with the solvent as the hydration layer changes Vh.
 
Benoit ''et al.'' showed that taking into account the hydrodynamic volume would solve the problem.  In his publication, Benoit showed that all synthetic polymers elutes on the same curve when the log of the intrinsic viscosity multiplied by the molar mass was plotted against the elution volume.  This is the basis of universal calibration which requires a viscometer to measure the intrinsic viscosity of the polymers.  Universal calibration was shown to work for branched polymers, copolymers as well as starburst polymers.
 
For good chromatography, there must be no interaction with the column other than that produced by size.  As the demands on polymer properties increased, the necessity of getting absolute information on the molar mass and size also increased. This was especially important in pharmaceutical applications where slight changes in [[molar mass]] (e.g. [[Particle aggregation|aggregation]]) or shape may result in different [[biological activity]]. These changes can actually have a harmful effect instead of a beneficial one.
 
To obtain molar mass, [[light scattering instruments]] need to measure the intensity of light scattered at zero angle.  This is impractical as the laser source would outshine the light scattering intensity at zero angle.  The 2 alternatives are to measure very close to zero angle or to measure at many angle and extrapolate using a model (Rayleigh, Rayleigh-Gans-Debye, Berry, Mie, etc.) to zero degree angle.
 
Traditional light scattering instruments worked by taking readings from multiple angles, each being measured in series. A low angle light scattering system was developed in the early 1970s that allowed a single measurement to be used to calculate the molar mass. Although measurements at low angles are better for fundamental physical reasons (molecules tend to scatter more light in lower angle directions than in higher angles), low angle scattering events caused by dust and contamination of the mobile phase easily overwhelm the scattering from the molecules of interest. When the low-angle laser light scattering (LALLS) became popular in the 1970s and mid-1980s, good quality disposable filters were not readily available and hence multi-angle measurements gained favour.
 
Multi-angle light scattering was invented in the mid-1980s and instruments like that were able to make measurements at the different angles simultaneously but it was not until the later 1980s (10-12) that the connection of [[multi-angle laser light scattering]] (MALS) detectors to SEC systems was a practical proposition enabling both molar mass and size to be determined from each slice of the polymer fraction.
 
== Applications ==
Light scattering measurements can be applied to [[synthetic polymer]]s, [[protein]]s, [[pharmaceuticals]] and particles such as [[liposome]]s, [[micelles]], and encapsulated proteins. Measurements can be made in one of two modes which are [[un-fractionated]] (batch mode) or in [[continuous flow]] mode (with SEC, HPLC or any other [[flow fractionation method]]). Batch mode experiments can be performed either by injecting a sample into a flow cell with a syringe or with the use of discrete vials. These measurements are most often used to measure timed events like [[antibody-antigen reactions]] or [[protein assembly]]. Batch mode measurements can also be used to determine the second virial coefficient (A2), a value that gives a measure of the likelihood of crystallization or aggregation in a given solvent. Continuous flow experiments can be used to study material eluting from virtually any source. More conventionally, the detectors are coupled to a variety of different chromatographic separation systems. The ability to determine the mass and size of the materials eluting then combines the advantage of the separation system with an absolute measurement of the mass and size of the species eluting.
 
The addition of an SLS detector coupled downstream to a chromatographic system allows the utility of SEC or similar separation combined with the advantage of an absolute detection method. The light scattering data is purely dependent on the light scattering signal times the concentration; the elution time is irrelevant and the separation can be changed for different samples without recalibration. In addition, a non-size separation method such as HPLC or IC can also be used.
As the light scattering detector is mass dependent, it becomes more sensitive as the molar mass increases. Thus it is an excellent tool for detecting aggregation. The higher the aggregation number, the more sensitive the detector becomes.
 
== Low Angle (Laser) Light Scattering (LALS) Method ==
 
LALS measurements are measuring at a very low angle where the scattering vector is almost zero. LALS does not need any model to fit the angular dependence and hence is giving more reliable molecular weights measurements for large molecules.  LALS alone does not give any indication of the root mean square radius.
 
== Multi Angle (Laser) Light Scattering (MALS) Method ==
 
MALS measurements work by calculating the amount of light scattered at each angle detected. The calculation is based on the intensity of light measured and the quantum efficiency of each detector. Then a model is used to approximate the intensity of light scattered at zero angle. The zero angle light scattered is then related to the molar mass.
 
As previously noted, the MALS detector can also provide information about the size of the molecule. This information is the Root Mean Square radius of the molecule (RMS or Rg). This is different from the Rh mentioned above who is taking the hydration layer into account. The purely mathematical root mean square radius is defined as the radii making up the molecule multiplied by the mass at that radius.
 
== Bibliography ==
*A. Einstein, Ann. Phys. 33 (1910), 1275
*C.V. Raman, Indian J. Phys. 2 (1927), 1
*P.Debye, J. Appl. Phys. 15 (1944), 338
*B.H. Zimm, J. Chem. Phys 13 (1945), 141
*B.H. Zimm, J. Chem. Phys 16 (1948), 1093
*B.H. Zimm, R.S. Stein and P. Dotty, Pol. Bull. 1,(1945), 90
*M. Fixman, J. Chem. Phys. 23 (1955), 2074
*A.C. Ouano and W. Kaye J. Poly. Sci. A1(12) (1974), 1151
*Z. Grubisic, P. Rempp, and H. Benoit, J. Polym. Sci., 5 (1967), 753
*Flow Through MALS detector, DLS 800, Science Spectrum Inc.
*P.J. Wyatt, C. Jackson and G.K. Wyatt Am. Lab 20(6) (1988), 86
*P.J. Wyatt, D. L. Hicks, C. Jackson and G.K. Wyatt Am. Lab. 20(6) (1988), 106
*C. Jackson, L.M. Nilsson and P.J. Wyatt J. Appl. Poly. Sci. 43 (1989), 99
 
[[Category:Chemical properties]]
[[Category:Mass]]

Latest revision as of 11:54, 5 May 2014

If you"re like me then you hate not having your mobile phone. As a result, I "d been looking for a small bag that I might wear all day at work, then take out in the evening, that was comfortable and fashionable at the same time. I took a look at lots of small purses and pouches but they all had issues. On some, the shoulder strap was too thin and lightweight and I understood it would quickly break. Others were the ideal size but simply weren"t stylish enough for my requirements. I truly care about how I look as I believe it"s a reflection of who I am. Check This Out At Amazon.Com/Bag Shoulder Guaranteed Shipping Accessories/Dp/B00 Nqc9 Zci/Cell Phone Pouch/ is a poetic online database for more about how to do this idea. So a practical option that wasn"t trendy too, just wasn"t going to work for me.

Then I discovered the Gracie Smart phone Holder from My Best Friend is a Bag, an Australian business that has just started offering on Amazon. It was love at first sight.

The Gracie is so pretty. It"s constructed of faux shiny leather with a spectacular Brushed Nickel cross body chain. Simply the correct amount of luster and fashionability for me. I couldn"t wait to try one and I started wearing it the minute it showed up from Amazon. I am truly happy with my purchase. I selected the Black Gracie (she comes in 3 colors, Red, Black and Silver) and have been using it every day at work and have actually even worn it out during the night. I"ve had a lot of compliments from good friends and colleagues which has actually been great however that"s not why I purchased it. I purchased it so I would always have my phone right by my side and it has actually made my life a lot simpler! I simply pop my phone into my Gracie very first thing in the morning and no matter where I am or what I"m doing, when that phone rings I"m there. I never ever miss out on a call or a message.

I"ve constantly been a big fan of Amazon. I really value the security that comes with buying from them with their refund warranty. This time too, I was so amazed with the follow up I got from My Best Friend is a Bag, they truly wanted me to be happy with my purchase and I am. On their listing they say that their products are Hand Made and it shows. I am so pleased with the quality of my Gracie.

If you"re in the marketplace for an attractive method to carry your cellphone, then you ought to give the Gracie a go. I encourage you to click the link below and order one.

They also make a wonderful present, so consider buying one for your Best Friend at the exact same time..

When you have almost any inquiries relating to wherever and how you can work with health blog, it is possible to contact us with our site.