Ionised concentrations in calcium and magnesium buffers: Standards and precise measurement are mandatory.

Prog Biophys Mol Biol

Medical, Veterinary and Life Sciences Faculty, University of Glasgow, G12 8QQ, UK.

Published: September 2016

AI Article Synopsis

  • In buffer solutions containing Ca(2+) and Mg(2+), measured or calculated ionized concentrations can differ significantly (by up to a factor of seven) due to inconsistencies in literature constants and measurement techniques.
  • There are issues such as the lack of consensus on tabulated constants, complexities in calculating ionic strength corrections, and inaccuracies in pH measurements, which hinder reliable determination of ion concentrations.
  • The Ligand Optimisation Method is highlighted as an accurate approach to measure the ionized concentrations, emphasizing the need for standardization in Ca(2+)/Mg(2+) buffers to enable reliable comparisons across different laboratories.

Article Abstract

In Ca(2+) and Mg(2+) buffer solutions the ionised concentrations ([X(2+)]) are either calculated or measured. Calculated values vary by up to a factor of seven due to the following four problems: 1) There is no agreement amongst the tabulated constants in the literature. These constants have usually to be corrected for ionic strength and temperature. 2) The ionic strength correction entails the calculation of the single ion activity coefficient, which involves non-thermodynamic assumptions; the data for temperature correction is not always available. 3) Measured pH is in terms of activity i.e. pHa. pHa measurements are complicated by the change in the liquid junction potentials at the reference electrode making an accurate conversion from H(+) activity to H(+) concentration uncertain. 4) Ligands such as EGTA bind water and are not 100% pure. Ligand purity has to be measured, even when the [X(2+)] are calculated. The calculated [X(2+)] in buffers are so inconsistent that calculation is not an option. Until standards are available, the [X(2+)] in the buffers must be measured. The Ligand Optimisation Method is an accurate and independently verified method of doing this (McGuigan & Stumpff, Anal. Biochem. 436, 29, 2013). Lack of standards means it is not possible to compare the published [Ca(2+)] in the nmolar range, and the apparent constant (K(/)) values for Ca(2+) and Mg(2+) binding to intracellular ligands amongst different laboratories. Standardisation of Ca(2+)/Mg(2+) buffers is now essential. The parameters to achieve this are proposed.

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http://dx.doi.org/10.1016/j.pbiomolbio.2016.03.002DOI Listing

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