Lecture #7 (2D NMR) Utility of Resonance Assignments



Similar documents
NMR Nuclear Magnetic Resonance

NMR Spectroscopy in Notre Dame

Nuclear Magnetic Resonance Spectroscopy

Signal Manipulation. time domain NMR signal in MHz range is converted to khz (audio) range by mixing with the reference ( carrier ) frequency

Proton Nuclear Magnetic Resonance Spectroscopy

13C NMR Spectroscopy

NMR for Physical and Biological Scientists Thomas C. Pochapsky and Susan Sondej Pochapsky Table of Contents

Tetramethylsilane (TMS) Trimethylsilyl d 4. -propionic acid (TMSP) Dioxane. O - Na + Dimethylfura n. Potassium Hydrogen Phthalate. Sodium Maleate CH 3

Generation and Detection of NMR Signals

Introduction to NMR spectroscopy. Swiss Institute of Bioinformatics I.Phan & J. Kopp

Organic Chemistry Tenth Edition

Introduction to Nuclear Magnetic Resonance (NMR) And. NMR Metabolomics

4. It is possible to excite, or flip the nuclear magnetic vector from the α-state to the β-state by bridging the energy gap between the two. This is a

Electronic Supplementary Information

Nuclear Magnetic Resonance Spectroscopy

Nuclear Magnetic Resonance (NMR) Spectroscopy cont... Recommended Reading:

NMR SPECTROSCOPY. Basic Principles, Concepts, and Applications in Chemistry. Harald Günther University of Siegen, Siegen, Germany.

PROTON NUCLEAR MAGNETIC RESONANCE SPECTROSCOPY (H-NMR)

Proton Nuclear Magnetic Resonance Spectroscopy

Determination of Equilibrium Constants using NMR Spectrscopy

Proton Nuclear Magnetic Resonance ( 1 H-NMR) Spectroscopy

BUILDING BLOCKS FOR MULTIDIMENSIONAL NMR AND SPECIAL CONSIDERATIONS FOR BIOLOGICAL APPLICATIONS OF NMR

The Four Questions to Ask While Interpreting Spectra. 1. How many different environments are there?

Structural Bioinformatics (C3210) Experimental Methods for Macromolecular Structure Determination

Nuclear Magnetic Resonance

Nuclear Magnetic Resonance (NMR) Spectroscopy

The Hydrogen Atom Is a Magnet.

NMR practice times. Mo pm Jim 2-4:30 Ning 4:30-7. Tues pm Jianing 2-4:30 Ting 4:30-7. Fri Donia 10-12:00 Ilya 2-4

Protein Dynamics by NMR. Why NMR is the best!

Determining the Structure of an Organic Compound

8.1 Relaxation in NMR Spectroscopy

Used to determine relative location of atoms within a molecule Most helpful spectroscopic technique in organic chemistry Related to MRI in medicine

Background A nucleus with an odd atomic number or an odd mass number has a nuclear spin that can be observed by NMR spectrometers.

Nuclear Magnetic Resonance notes

Lecture 15: Enzymes & Kinetics Mechanisms

Spin-Lattice Relaxation Times

Basic Principles of Magnetic Resonance

Proton NMR. One Dimensional H-NMR. Cl S. Common types of NMR experiments: 1-H NMR

Chapter 11 Structure Determination: Nuclear Magnetic Resonance Spectroscopy. Nuclear Magnetic Resonance Spectroscopy Nuclear Magnetic Resonance

NMR Signal Properties & Data Processing

NMR SPECTROSCOPY A N I N T R O D U C T I O N T O... Self-study booklet NUCLEAR MAGNETIC RESONANCE δ PUBLISHING

Determination of Molecular Structure by MOLECULAR SPECTROSCOPY

Infrared Spectroscopy 紅 外 線 光 譜 儀

How To Understand The Measurement Process

Trans Fats. What is a trans fat? Trans fatty acids, or trans fats as they are known, are certain

NMR - Basic principles

Chapter 13 Spectroscopy NMR, IR, MS, UV-Vis

Chapter 1. Fundamentals of NMR THOMAS L. JAMES. Department of Pharmaceutical Chemistry University of California San Francisco, CA U.S.A.

Amino Acids. Amino acids are the building blocks of proteins. All AA s have the same basic structure: Side Chain. Alpha Carbon. Carboxyl. Group.

Infrared Spectroscopy: Theory

Nuclear Magnetic Resonance Spectroscopy

Molecular Models in Biology

Introduction to Nuclear Magnetic Resonance Spectroscopy

Practical guide for quantitative 1D NMR integration Eugenio Alvarado, University of Michigan, 05/10/10

For example: (Example is from page 50 of the Thinkbook)

Supporting Information

The Experiment Some nuclei have nuclear magnetic moments; just as importantly, some do not

Time out states and transitions

Chemical Exchange in NMR Spectroscopy

Solving Spectroscopy Problems

NUCLEAR MAGNETIC RESONANCE. Advanced Laboratory, Physics 407, University of Wisconsin Madison, Wisconsin 53706

Nuclear Magnetic Resonance Spectroscopy

INFRARED SPECTROSCOPY (IR)

Basic NMR Concepts: A Guide for the Modern Laboratory

NMR Techniques Applied to Mineral Oil, Water, and Ethanol

NMR Spectroscopy. Applications. Drug design MRI. Food quality. Structural biology. Metabonomics

INTRODUCTION TO CHEMICAL EXCHANGE WITH THE MEXICO PROGRAM

GE Medical Systems Training in Partnership. Module 8: IQ: Acquisition Time

1 Introduction to NMR Spectroscopy

Nuclear Magnetic Resonance and Its Application in Condensed Matter Physics

Nuclear Shielding and 1. H Chemical Shifts. 1 H NMR Spectroscopy Nuclear Magnetic Resonance

Pulsed Fourier Transform NMR The rotating frame of reference. The NMR Experiment. The Rotating Frame of Reference.

Nuclear Magnetic Resonance (NMR) Wade Textbook

NMR and other Instrumental Techniques in Chemistry and the proposed National Curriculum.

8.2 The Nuclear Overhauser Effect

ph: Measurement and Uses

Chemistry 307 Chapter 10 Nuclear Magnetic Resonance

Prof.M.Perucca CORSO DI APPROFONDIMENTO DI FISICA ATOMICA: (III-INCONTRO) RISONANZA MAGNETICA NUCLEARE

Molecular Spectroscopy

m/z

18.2 Comparing Atoms. Atomic number. Chapter 18

Determination of Equilibrium Constants using NMR Spectroscopy

Signal to Noise Instrumental Excel Assignment

Nuclear Magnetic Resonance and the Measurement of Relaxation Times of Acetone with Gadolinium

Chapter 19 Nuclear Magnetic Resonance Spectroscopy (NMR)

Peptide bonds: resonance structure. Properties of proteins: Peptide bonds and side chains. Dihedral angles. Peptide bond. Protein physics, Lecture 5

E. K. A. ADVANCED PHYSICS LABORATORY PHYSICS 3081, 4051 NUCLEAR MAGNETIC RESONANCE

NMR Spectroscopy of Aromatic Compounds (#1e)

The Fundamentals of Infrared Spectroscopy. Joe Van Gompel, PhD

The Unified Scale for Referencing in NMR: New IUPAC Recommendations revised (cgf): 26 July 2010

(c) How would your answers to problem (a) change if the molecular weight of the protein was 100,000 Dalton?

Advanced Medicinal & Pharmaceutical Chemistry CHEM 5412 Dept. of Chemistry, TAMUK

Acids and Bases. but we will use the term Lewis acid to denote only those acids to which a bond can be made without breaking another bond

Pulsed Nuclear Magnetic Resonance An Experiment for UCSB s Advanced Laboratory

Chem101: General Chemistry Lecture 9 Acids and Bases

Understanding Precessional Frequency, Spin-Lattice and Spin-Spin Interactions in Pulsed Nuclear Magnetic Resonance Spectroscopy Introduction Theory

ELECTRONIC SUPPLEMENTARY INFORMATION

Spin-lattice and spin-spin relaxation

Transcription:

Lecture #7 (2D NMR) Basics of multidimensional NMR (2D NMR) 2D NOESY, COSY and TOCSY 2/23/15 Utility of Resonance Assignments Resonance Assignments: Assignment of frequency positions of resonances (peaks) in the NMR spectrum to specific atoms in the macromolecule. Macromolecule H Protein folding Resonance Assignments Dynamics (10-12 to seconds time scale) 1D 1H NMR spectrum Protein pka measurements Mapping ligand binding surfaces (drug discovery) Multidimensional experiments required to resolve peak overlap Structure 1

COSY: COrrelation SpectroscopY 2

Basic 2D COSY COSY: COrrelation SpectroscopY Review: the effect of 90 o pulses applied on different axes Before After o 90 o x pulse (B1) B 1 Bo Bo Mo Mo z x Detected component The amount of component in transverse plane is Mo sin (360* *t1) (Blue). Only this component is detected. Similar to 1D it will rotate in the transverse (xy) plane at a frequency 3

Peak Peak height proportional to: Mo sin (360 t 1 ) z F2 frequency domain x t 1 = 0 sec interferogram intensity Magnitude of peak maxima oscillates at sin (360* a*t 1 ) 4

Amplitude of peak is modulated by Cos (2 * a *t 1 ) Interferogram (the 2 nd ) a (direct dimension) a a 5

Case II (transfer during mixing period) t1 (F1) t2 (F2) Key experimental parameters for multidimensional NMR experiments (1) Sweep-width in indirect dimension: Controlled by the amount the t1 delay is incremented between successive experiments. (t 1 ): Amount that the t1 delay is incremented between successive experiments. SW(F1) = 1/( (t 1 )) ***Note: it s more complicated than this!! It depends upon how the experiment was performed. There are many ways to obtain quadrature detection in the indirect dimension (different ways to sample the signal so as to discern positive and negative frequencies in the indirect dimension). In these different methods (STATES, STATES-TPPI, TPPI, ECHO-ANTIECHO) the delay is not always incremented on each successive t1 increment! (t 1 )= 100 s t 1 =0 s Example: (t1)= 100 s 1 / (100 s) = 10,000Hz t 1 =100 s t 1 =200 s t 1 =300 s SW(F1) = 10,000Hz F2 (direct dimension) F1 (indirect dimension) t 1 =400 s (t 1 )= 50 s t 1 =0 s Example: (t1)= 50 s 1 / (50 s) = 20,000Hz t 1 =50 s t 1 =100 s t 1 =150 s SW(F1) = 20,000Hz F1 (indirect dimension) t 1 =200 s F2 (direct dimension) 6

(2) Digital resolution (DR) in indirect dimension Interferogram The more t 1 increments you collect the better the digital resolution in the indirect dimension. interferogram (t 1 ) 128 t1 increments 512 t1 increments Nyquist theorem: To properly determine the frequency of an oscillating signal must sample it at least twice per wavelength Typically 256 to 1024 experiments (increments) are recorded depending on the desired digital resolution in indirect dimension 7

(2) Digital resolution (DR) in indirect dimension A Indirect dimension (F2) Indirect dimension (F2) B Example: SW(F1) = 10,000 Hz expts. recorded = 128 DR= 156.3 Hz/point 128 1D files (serial files) collected in t1 dimension Example: SW(F1) = 10,000 Hz expts. recorded = 512 DR = 39.1 Hz/point 512 1D files (serial files) collected in t1 dimension Mid-80s Early 90s late 90s - to present Different strategies to assign proteins Homonuclear Methods (1H 2D COSY, TOCSY etc.) Proteins < 10-15 kd (< ~100 aa) Old School Triple Resonance (3D/4D 1H, 13C & 15N) (most common) Quadruple Resonance (3D/4D 1H, 13C & 15N) Proteins < 30 kd (< 250 aa) Proteins < 85 kd (< 723aa) JACS (2002) 124:10025-35. Direct dimension (F2) 8

Important 2D experiments used in homonuclear assignment methods 2D COSY 2D NOESY 2D COSY 2D TOCSY NOESY (Nuclear Overhauser Enhancement SpectroscopY): Connects hydrogen atom that are separated by < 5 Angstroms (<0.5nanometers) TOCSY (TOtal Correlation SpectroscopY): Connects hydrogen atoms that are part of the same spin network (spin system). Some people refer to this as a HOHAHA experiment. COSY (COrrelation SpectroscopY): Connects hydrogen atoms that are separated by three bonds or less *Homonuclear: Frequency of single atom type (hydrogen in these experiments) is observed in frequency dimensions In the COSY experiment, magnetization is transferred by scalar coupling. Protons that are more than three chemical bonds apart give no cross signal because the 4 J coupling constants are close to 0. Therefore, only signals of protons which are two or three bonds apart are visible in a COSY spectrum (red signals). The cross signals between HN and Halpha protons are of special importance because the phi torsion angle of the protein backbone can be derived from the 3 J coupling constant between them. 9

2D TOCSY 2D NOESY In the TOCSY experiment, magnetization is dispersed over a complete spin-system (set of hydrogen atoms) of an amino acid by successive scalar coupling. The TOCSY experiment correlates all protons of a spin system. Therefore, not only the red signals are visible (which also appear in a COSY spectrum) but also additional signals (green) which originate from the interaction of all protons of a spin system that are not directly connected via three chemical bonds. In the NOESY experiment, magnetization is transferred between 1H nuclei when they are < ~5A apart The closer the nuclei the stronger the cross-peak (proportional r -6 ) 10

Example 2D NOESY spectrum 1 mm Protein dissolved in water (55.5M H2O) 2D NOESY Experiment (transfer of magnetization via dipole-dipole interactions) H I 1D spectrum <6 angstroms H S < 5A Ha Hb (f) (g) < 5A Hc (a) (b) (c) (d) (e) I S 0 Hz frequency Example of single increment in the experiment (a) IS (b) (c) I cos (360* S *t 1 ) S I S Hb Hc Ha F2 F1 F2 (ppm) F1 (ppm) (d) I S m period (e) I S Non-equilibrium condition. Populations of S-spin inverted Transient NOE condition. Spin S has been inverted, while spin I has not. Hc Hb F2 Ha F1 NOE effect causes intensity of I to be reduced (negative NOE). The amount of S on z axis depends on cos (360* S *t 1 ). ( its projection onto the Y axis at step (c)) Therefore the intensity reduction in I is modulated by cos (360* S *t 1 ). Wo Assuming Negative NOE (Wo dominates) 11

2D NOESY Experiment (transfer of magnetization via dipole-dipole interactions) (f) H I 1D spectrum <6 angstroms H S Intensity of cross-peak related to mixing time (t m ) (a) (b) (c) (d) (e) I S 0 Hz frequency (d) (f) I S m period (e) I S Intensity of I modulated by amount of S magnetization at beginning of mixing time that is inverted. This in turn depends upon larmor frequency of spin S in t1 dimension. Therefore frequency of S nucleus in F1 dimension has been encoded within the amplitude of spin I when it is detected Rate of build-up of cross-peak is inversely proportional to distance separation S Direct detection of I oscillating at frequency I I Rate of NOE build-up (t2 -> F2) (t1 -> F1) I F2 (direct dimension) S F1 (indirect dimension) 50-200 ms Typical Mixing time We record NOESY spectra at a fixed tm value where intensity is proportional in inter-hydrogen atom separation (r IS ) 12

The sign of the cross-peak in NOESY depends on the molecular tumbling time (size) of the molecule or whether it is caused by chemical exchange. Large molecule (- NOE) Biomolecules! Wo dominates I F2 (direct dimension) S F1 (indirect dimension) Small molecule ( NOE) - I F2 (direct dimension) - H I S F1 (indirect dimension) r IS H S Cross-peaks from NOEs Protein requirements for homonuclear resonance assignment methods (1) Protein molecular weight < 10-15 kds (<~100aa) homonuclear assignment methods don t work for larger proteins because: (a) Increased spectral complexity. (signal overlap) (b) Increased proton transverse relaxation (smaller T 2 values cause proton magnetization to decay too rapidly. Important homonuclear proton COSY and TOCSY experiments no longer work ) (2) protein concentration > 0.25 to 0.5mM. Data collection for less concentrated proteins takes too long. S/N is proportional to Sqrt (# of scans). 16 times as many scans need to be acquired on a 0.125mM sample to get the same S/N ratio as obtained when the same experiment is acquired on the same sample concentrated to 0.5mM. (3) Salt (NaCl or KCl) concentrations <500mM Higher salt concentrations degrade the performance of the NMR probe reducing signal to noise. (4) Must not significantly aggregate. Aggregation increases apparent c. This decreases the T2 values. Cross-peaks from chemical exchange a Chemical exchange: During the mixing time ( m) the magnetic environment of hydrogen atom changes (chemical shift changes) as a result of conformational rearrangement or chemical reaction b F1 (indirect dimension) e.g. a b Conformational change (5) dissolved in non-protonated solvents. Protonated solvents give rise to signals in the NMR spectra that mask those of the protein. Note: Most experiments are performed on samples containing water which gives rise to a water peak at ~4.76ppm. This huge signal is normally eliminated by using water suppression techniques during the experiment (e.g. selective excitation, solvent presaturation, magnetic field gradients) Some good NMR buffers: (a) 50mM PO 4 /100mM NaCl/7% 2 H 2 O (D 2 O) (b) 50mM Tris-d11/100mM NaCl/7% 2 H 2 O (D 2 O) (c) deuterated acetate/100mm NaCl/7% 2 H 2 O (D 2 O) Frequently 0.01% Sodium Azide is also added to prevent microbial growth F2 (di t di i ) 13

Why do we need 2 H 2 O in the solvent? The magnetic field generated by the superconducting magnet changes with time ( drifts ) 2 H 2 O is used to lock the magnetic field (keep it from changing) during data acquisition On a 500 MHz NMR magnet 1 H frequency = 500 MHz 2 H frequency = 76.8 MHz (6) Sample should be soluble at ph values < 8.0 At alkaline ph values have increased rate of exchange of protein hydrogen atoms with solvent. This tends to attenuate the signals arising from exchangeable atoms. Solvent Exchange H A N H B O H C k intr H B N H A O acid or base catalyzed H C H B H A N H B (-) (-) O O N H C H A H C Example of base catalyzed NMR Experiment Lock System H A N Observed chem. shift of H A ~ chem. shift of H 2 O H 2 O 1H RF excitation & detection (500 MHz) 2 H RF excitation & detection (76.8MHz) Computer (signal processing and storage) Automatically adjust magnetic field to counter-act field drift Monitor 2 H Signal position Chemical shift of atom H A = P H A N Fraction of N-H A ~10-3 M A P O H A H H 2 O B ~ H 2 O Fraction of H A -O-H B ~55 M 14

Protons that exchange H N Backbone amide Trp indole His sidechain Sample manipulation trick: Change buffer into D 2 O solvent to simplify the NMR spectra H H O H H O H H O O H Ser/Thr/Tyr Arginine sidechain N-term residue, Lys sidechain O C.. S H.. HO Carboxylic acid (C-term residue, Asp, Glu) Asn, Gln sidechain Cys sidechain N-term.. N C C N C C N C C.. CH CH HO CH 3 H 3 C CH 3 Buffer exchange protein into 100% D 2 O solvent (cycle to higher ph to facilitate exchange: ph <7 ph 8 ph <7 ) H C-term water sample 50mM PO 4 100mM NaCl 7% 2 H 2 O (D 2 O) 0.01% NaN 3 Not observable in NMR spectrum D H O D H O D H O N-term.. N C C N C C N C C.. C-term CH CH DO CH 3 H 3 C CH 3 H D2O sample 50mM PO 4 100mM NaCl 99.99% 2 H 2 O (D 2 O) 0.01% NaN 3 15

2026 © DocPlayer.net Privacy Policy | Terms of Service | Feedback  | Do Not Sell My Personal Information