Q.99 Which of the following techniques is/are used for determining the
three–dimensional structure of proteins?
(A) Cryo–electron Microscopy
(B) Circular Dichroism
(C) Nuclear Magnetic Resonance Spectroscopy
(D) X–ray Diffraction

Cryo-electron Microscopy, Nuclear Magnetic Resonance Spectroscopy, and X-ray Diffraction directly determine the three-dimensional structure of proteins at atomic resolution, making options (A), (C), and (D) correct. Circular Dichroism primarily analyzes secondary structure content rather than full 3D atomic models. The correct answer for this CSIR NET question is (A), (C), and (D), as multiple techniques apply.​

Option Analysis

Cryo-Electron Microscopy (A)
Cryo-EM images frozen protein samples to reconstruct 3D structures without crystallization, excelling for large complexes and membrane proteins at resolutions below 3 Å. Recent advances extend it to smaller proteins via scaffolds.​

Circular Dichroism (B)
CD spectroscopy measures differential light absorption to estimate secondary structure percentages like α-helices and β-sheets from far-UV spectra, but lacks atomic 3D positioning. Near-UV CD probes tertiary environments indirectly, not full structures.​

NMR Spectroscopy (C)
NMR uses magnetic nuclei interactions in solution to derive 3D coordinates via distance restraints and angles, ideal for dynamics in proteins up to ~50 kDa.​

X-ray Diffraction (D)
X-ray crystallography analyzes diffraction from protein crystals to map atomic positions at high resolution, the gold standard for precise structures.​

Technique Comparison

CSIR NET Relevance

These methods appear frequently in structural biology sections, emphasizing atomic-level 3D determination over secondary structure tools like CD. Cryo-EM’s rise complements traditional X-ray and NMR for competitive exam contexts.​