NMR determined Rotational correlation time: Difference between revisions

Revision as of 18:23, 16 December 2009

Brownian rotation diffusion of a particle in solution has a characteristic time constant called rotational correlation time (τ_c). It is the time it takes the particle to rotate by one radian and it depends on the particle size. For globular proteins a spherical approximation can be used and the rotational correlation time is given by Stoke's law

<math>\tau_c=\frac{4\pi\eta r^3}{3kT}</math>,

where <math>\eta</math> is the viscosity of the solvent, <math>r</math> is the effective hydrodynamic radius of the protein molecule, <math>k</math> is the Boltzmann constant and <math>T</math> is the temperature. The hydrodynamic radius can be estimated from the molecular weight of the protein (M) as

<math>r\approx\sqrt[3]{\frac{3M}{4\pi\rho N_a}}+r_w</math>,

where <math>\rho</math> is the average density for proteins (1.37 g/cm3), <math>N_a</math> is the Avogadro's number and <math>r_w</math> is the hydration radius (1.6 to 3.2 A)^[1]. As a general rule of thumb, the τ_c of a monomeric protein in solution in nanoseconds is approximately 0.6 times its molecular weight in kDa.

For rigid protein molecules, in the limit of slow molecular motion (τ_c >> 0.5 ns) and high magnetic field (500 MHz or greater), a closed-form solution for τ_c as a function of the ratio of the longitudinal (T₁) and transverse (T₂) ¹⁵N relaxation times exists:

<math>\tau_c\approx\frac{1}{4\pi\nu_N}\sqrt{6\frac{T_1}{T_2}-7}</math>,

where ν_N is the ¹⁵N resonance frequency (in Hz). This equation is derived from Eq. 8 in ^[2] by considering only J(0) and J(ωN) spectral density terms and neglecting higher frequency terms.

Average ¹⁵N T₁ and T₂ relaxation times for a given protein can be measured using 1D ¹⁵N-edited relaxation experiments ^[3]. To minimize contributions from unfolded segments each 1D spectum is integrated over the downfield backbone amide ¹H region (typically 10.5 to 8.5 ppm) and the results are used to fit an exponential decay as a function of delay time. One then computes the correlation time using Eq. 3, and compares it to a standard curve of τ_c vs. protein molecular weight (MW) obtained at the same temperature on a series of known monomeric proteins of varying size. The T1-over-T2 approach is reliable for proteins up to MW ≈ 25 kDa, where accurate measurement of the diminishing ¹⁵N T₂ becomes problematic.

Protocols for Bruker and Varian NMR Instruments

References

↑ Cavanagh J., Fairbrother W.J., Palmer, A.G, Rance M., Skelton N.J. (2007) Protein NMR Spectroscopy: Principles and Practice, p21, Elsevier
↑ Kay, L.E., Torchia, D.A. and Bax, A. (1989) Backbone dynamics of proteins as studied by ¹⁵N inverse detected heteronuclear NMR spectroscopy: Application to staphylococcal nuclease. Biochemistry, 28, 8972-8979.
↑ Farrow, N.A., Muhandiram, R., Singer, A.U., Pascal, S.M., Kay, C.M., Gish, G., Shoelson, S.E., Pawson, T., Forman-Kay, J.D. and Kay, L.E. (1994) Backbone dynamics of a free and phosphopeptide-complexed Src homology 2 domain studied by ¹⁵N NMR relaxation. Biochemistry, 33, 5984-6003.

-- JimAramini - 10 Nov 2009

[1] Cavanagh J., Fairbrother W.J., Palmer, A.G, Rance M., Skelton N.J. (2007) Protein NMR Spectroscopy: Principles and Practice, p21, Elsevier

[2] Kay, L.E., Torchia, D.A. and Bax, A. (1989) Backbone dynamics of proteins as studied by ¹⁵N inverse detected heteronuclear NMR spectroscopy: Application to staphylococcal nuclease. Biochemistry, 28, 8972-8979.

[3] Farrow, N.A., Muhandiram, R., Singer, A.U., Pascal, S.M., Kay, C.M., Gish, G., Shoelson, S.E., Pawson, T., Forman-Kay, J.D. and Kay, L.E. (1994) Backbone dynamics of a free and phosphopeptide-complexed Src homology 2 domain studied by ¹⁵N NMR relaxation. Biochemistry, 33, 5984-6003.

[1]

[2]

[3]

@@ Line 1: / Line 1: @@
-== '''Introduction'''  ==
+Brownian rotation diffusion of a particle in solution has a characteristic time constant called rotational correlation time (τ<sub>c</sub>). It is the time it takes the particle to rotate by one radian and it depends on the particle size. For globular proteins a spherical approximation can be used and the rotational correlation time is given by Stoke's law
-The rotational correlation time of a protein in solution is the time for a protein to rotate one radian. In the limit of slow molecular motion (τ<sub>c</sub> &gt;&gt; 0.5 ns), the correlation time of a protein is related to the ratio of the longitudinal (T<sub>1</sub>) and transverse (T<sub>2</sub>) <sup>15</sup>N relaxation times, and nuclear frequency (ν<sub>N</sub>) according to Eq. 1, which is derived from Eq. 8 in Kay et al. (Ref. 1) by considering only J(0) and J(ω) spectral densities and neglecting higher frequency terms.&nbsp;&nbsp;&nbsp;&nbsp;&nbsp; &nbsp;&nbsp;&nbsp; [[Image:Tc eq1.png|center|250x50px]]
+<math>\tau_c=\frac{4\pi\eta r^3}{3kT}</math>,
-<br>
+where <math>\eta</math> is the viscosity of the solvent, <math>r</math> is the effective hydrodynamic radius of the protein molecule, <math>k</math> is the Boltzmann constant and <math>T</math> is the temperature. The hydrodynamic radius can be estimated from the molecular weight of the protein (M) as
-In practice, global <sup>15</sup>N T<sub>1</sub> and T<sub>2</sub> relaxation times for an unknown protein target can be obtained on Bruker or Varian NMR sytems using 1D <sup>15</sup>N-edited relaxation experiments (Ref. 2), by fitting integrated signal in the backbone amide <sup>1</sup>H region of the spectrum as a function of delay time to an exponential decay. One then computes the correlation time using Eq. 1, and compares it to a standard curve of τ<sub>c</sub> vs. protein molecular weight (MW) obtained at the same temperature on a series of known monomeric proteins of varying size.&nbsp; As a general rule of thumb, the τ<sub>c</sub> of a monomeric protein in solution in nanoseconds is approximately 0.6 times its molecular weight in kiloDaltons. This approach is reliable up to MW ≈ 25 kDa, where accurate measurement of the diminishing <sup>15</sup>N T<sub>2</sub> becomes problematic.&nbsp;<br>
+<math>r\approx\sqrt[3]{\frac{3M}{4\pi\rho N_a}}+r_w</math>,
+where <math>\rho</math> is the average density for proteins (1.37 g/cm3), <math>N_a</math> is the Avogadro's number and <math>r_w</math> is the hydration radius (1.6 to 3.2 A)<ref>Cavanagh J., Fairbrother W.J., Palmer, A.G, Rance M., Skelton N.J. (2007) Protein NMR Spectroscopy: Principles and Practice, p21, Elsevier</ref>. As a general rule of thumb, the τ<sub>c</sub> of a monomeric protein in solution in nanoseconds is approximately 0.6 times its molecular weight in kDa.
+For rigid protein molecules, in the limit of slow molecular motion (τ<sub>c</sub> &gt;&gt; 0.5 ns) and high magnetic field (500 MHz or greater), a closed-form solution for τ<sub>c</sub> as a function of the ratio of the longitudinal (T<sub>1</sub>) and transverse (T<sub>2</sub>) <sup>15</sup>N relaxation times exists:
+<math>\tau_c\approx\frac{1}{4\pi\nu_N}\sqrt{6\frac{T_1}{T_2}-7}</math>,
+where ν<sub>N</sub> is the <sup>15</sup>N resonance frequency (in Hz). This equation is derived from Eq. 8 in <ref>Kay, L.E., Torchia, D.A. and Bax, A. (1989) Backbone dynamics of proteins as studied by <sup>15</sup>N inverse detected heteronuclear NMR spectroscopy: Application to staphylococcal nuclease. ''Biochemistry'', '''28''', 8972-8979.</ref> by considering only J(0) and J(ωN) spectral density terms and neglecting higher frequency terms.
+Average <sup>15</sup>N T<sub>1</sub> and T<sub>2</sub> relaxation times for a given protein can be measured using 1D <sup>15</sup>N-edited relaxation experiments <ref>Farrow, N.A., Muhandiram, R., Singer, A.U., Pascal, S.M., Kay, C.M., Gish, G., Shoelson, S.E., Pawson, T., Forman-Kay, J.D. and Kay, L.E. (1994) Backbone dynamics of a free and phosphopeptide-complexed Src homology 2 domain studied by <sup>15</sup>N NMR relaxation. ''Biochemistry'', '''33''', 5984-6003.</ref>. To minimize contributions from unfolded segments each 1D spectum is integrated over the downfield backbone amide <sup>1</sup>H region (typically 10.5 to 8.5 ppm) and the results are used to fit an exponential decay as a function of delay time. One then computes the correlation time using Eq. 3, and compares it to a standard curve of τ<sub>c</sub> vs. protein molecular weight (MW) obtained at the same temperature on a series of known monomeric proteins of varying size. The T1-over-T2 approach is reliable for proteins up to MW ≈ 25 kDa, where accurate measurement of the diminishing <sup>15</sup>N T<sub>2</sub> becomes problematic.
 == <span class="mw-headline">'''Protocols for Bruker and Varian NMR Instruments'''</span> ==
@@ Line 14: / Line 25: @@
 == <span class="mw-headline">'''References'''  </span>  ==
-.&nbsp;&nbsp;&nbsp; Kay, L.E., Torchia, D.A. and Bax, A. (1989) Backbone dynamics of proteins as studied by <sup>15</sup>N inverse detected heteronuclear NMR spectroscopy:&nbsp; Application to staphylococcal nuclease. ''Biochemistry 28'', 8972-8979.<br>2.&nbsp;&nbsp;&nbsp; Farrow, N.A., Muhandiram, R., Singer, A.U., Pascal, S.M., Kay, C.M., Gish, G., Shoelson, S.E., Pawson, T., Forman-Kay, J.D. and Kay, L.E. (1994) Backbone dynamics of a free and phosphopeptide-complexed Src homology 2 domain studied by <sup>15</sup>N NMR relaxation. ''Biochemistry 33'', 5984-6003.<br>
+<references/>
-<br>
 -- JimAramini - 10 Nov 2009

NMR determined Rotational correlation time: Difference between revisions

Revision as of 18:23, 16 December 2009

Protocols for Bruker and Varian NMR Instruments

References

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