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Unit 5.2 & 5.5
Biochemical network mapping
(MetaMapp)
Dinesh Barupal
dinkumar@ucdavis.edu
DATA
ACQUISITION
Separation
Detection
SAMPLING
EXTRACTION
DATA
PROCESSING
File Conversion
Baseline Correction
Peak Detection
Deconvolution
Adduct Annotation
Alignment
Gap Filling
STATISTICS
Normalization
Multivariate Analysis
(Parametric, Nonparametric)
Univariate Analysis
(Unsupervised, Supervised)
BIOLOGICAL
INTERPRETATION
Pathway Mapping
Network Enrichment
STUDY DESIGN
VALIDATION
COMPOUND
IDENTIFICATION
Molecular Formula ID
Structure ID
MS Library Search
Database Search
In silico Fragmentation
WCMC
UC Davis
Questions :
• Why a network graph ?
• How to create biochemical network map of
identified metabolites ?
• How to include all the identified metabolites into a
network ?
• How to visualize and make publication ready
network graphs ?
• How to use MetaMapp and Cytoscape software ?
What is a network graph ?
A network graph represents entities as nodes (dots) and various
relationships among them as edges (links).
A
C
D
B
E
relationship X
An example network graph
Nodes can be – genes, proteins, reactions, metabolites.
Edges can be – correlation, reactions, reaction pairs,
pathways, chemical similarity, mass spectral similarity.
Edges can have direction like A B or B A.
Notable examples –
Air transportation network
Citation/ co-author network
Social network
Metabolic network
http://bmcgenomics.biomedcentral.com/articles/10.1186/1471-2164-13-334
What is a metabolic network ?
Tools for make this type of network
are –
• MetScape (http://metscape.ncibi.org/)
• MetaBox
(www.metabox.fiehnlab.ucdavis.edu)
• KEGG spider
(https://genomebiology.biomedcentral
.com/articles/10.1186/gb-2008-9-12-
r179)
• CPDB (http://consensuspathdb.org/)
• MetExplore
(http://metexplore.toulouse.inra.fr)
A
C
D
B
E
reaction X
A metabolite
Not every detected metabolite will be included in this network.
Two representations of the EC 2.3.1.35 reaction.
Two ways to convert a reaction to a graph
The KEGG RPAIR database is a manually curated
collection of reactant pairs (substrate-product pairs)
and chemical structure transformation patterns in
enzymatic reactions.
Masanori Arita PNAS 2004;101:1543-1547
Connect only the actual subtract-product and ignore the side
product or co-factors.
Biochemical databases provide list of metabolites and reactions among them.
An example of a metabolic reaction :
http://www.brenda-enzymes.org/ http://www.genome.jp/kegg/ https://metacyc.org/ http://www.reactome.org/
Major DBs that provided curated list of biochemical reactions.
Glucose-
6P
D-Glucose
D-Glucose 6-phosphate + H2O <=> D-Glucose + Orthophosphate
http://www.genome.jp/dbget-bin/www_bget?rn:R00303
~ 25000 metabolic reactions are known for various organisms.
Node A Node B
Node A Edge Node B
Cpd 1 KEGG Cpd 2
Cpd 3 KEGG Cpd 4
Cpd 4 KEGG Cpd 5
Cpd 6 KEGG Cpd 7
… KEGG …
Metabolic network in a text format
How to make a metabolic network ?
A
C
D
B
E
reaction X
A metabolite
But not all the metabolites have reaction annotations ?
https://bmcbioinformatics.biomedcentral.com/articl
es/10.1186/1471-2105-13-99
https://www.nature.com/articles/s41598-017-15231-w
Many significant (p<0.05) compounds are
not present in pathway databases
What is a chemical similarity coefficient ?
A
C
D
B
E
Chemical similarity
A metabolite
Xanthine Hypoxanthine
Tanimoto Chemical
Similarity score
0.917
Tanimoto = AB / ( A + B - AB )
Substructure decomposition for calculations of chemical similarity
http://www.pnas.org/content/106/40/17187
What is a MetaMapp network ?
All the identified
metabolites are
included in the
graph.
What is MetaMapp ?
MetaMapp: mapping and visualizing metabolomic data by integrating information from biochemical pathways and chemical and
mass spectral similarity https://bmcbioinformatics.biomedcentral.com/articles/10.1186/1471-2105-13-99
MetaMapp is a approach to map all the detected metabolites into a network
graph that resembles known biochemistry
Available at metamapp.fiehnlab.ucdavis.edu
Input file :
MetaMapp R-
Package (openCPU
version)
Network file
Node attribute file
How to use MetaMapp ?
How to get SMILES codes ?
How to use MetaMapp ?
Prepare the input file.
• This is the minimum input
• No duplicate CIDs are allowed
Example :
spring_2018_metabolomics_course_metamapp_
example.xlsx
About the example dataset
• Comparison of the plasma metabolome in
Non alcoholic fatty liver disease subjects and
the controls.
• HILIC + CSH assays
• ~ 650 identified metabolites.
• Unpublished (you can write a paper out of it).
MetaMapp input file errors -
• Duplicate PubChem CIDs
• Duplicate names
• Missing SMILES codes
• Missing p-value or fold-change
• Headers mismatch
• > 1000 compounds
How to use MetaMapp ?
Obtaining the MetaMapp files.
• Go to http://metamapp.fiehnlab.ucdavis.edu
Copy and paste your data
in this box
Click here
Now, click on these two buttons
chemsim_krp_07.sif node_attributes_chemsim_krp_07.tsv
Both files are provided in the example folder for the case study.
chemsim_krp_07.sif
node_attributes_chemsim_krp_07.tsv
Structure of the created files.
Both files will be imported in the Cytoscape
software for visualization
KRP – KEGG Reaction Pairs – biochemical relationships
TMSIM – Tanimoto similarity – chemical relationships
What is Cytoscape ?
The most used network visualization and
analysis tool.
http://journals.plos.org/plosbiology/article?id=10.1371%2Fjournal.pbio.1001843http://www.cytoscape.org/
Backed by strong institutions
Visualize a range of experimental data on a
network graph
Useful graph layout algorithms
Graph theory calculations
Easy organization of multiple networks for
comparisons.
Faster navigation of large networks
Filter and query the network
Contributed plugins
Works on PC, Max and Linux system
USB drive contains a copy of Cytoscape software
Cytoscape basic features
Click here
Start Cytoscape software
Locate the chemsim_krp_07.sif file and click import.
The file shall be in your download folder or you can use
the file in the example folder.
How to use Cytoscape?
Import a new network
If you want to import a new network file in already running Cytoscape
Select the .sif file
Visualization panel
Table panel highlights the data related to selected node
(yellow).
Cytoscape windwos
Show graphics details
Tip: if you don’t see the labels/edges/shapes/colors in graph, click on “Show graphics details”.
Visualize using the yFiles (organic layout). You can try other layout methods, but this one is
recommended.
Layout a network graph
Network graph after organic layout
Now import your Node Attributes file
Import your Node Attributes file
Import your Node Attributes file
“Key” symbol
should be
PubChem_ID
Import your Node Attributes file
Table panel after importing the node attributes.
Data visualization
All visual properties
can be accessed in the
style tab.
Node color
Node size
Node label
Node label position
Node Label font size
Edge color
Edge width
Network background color
Change network background color
1
2
3
Select black background color or any color you like.
Double click here
click here
Node coloring : “Node Fill color”
Red = higher
Blue = lower
Yellow = no
change
Node coloring : “Node Fill color”
Change node label
You can choose any
label from the node
attribute file.
You need to zoom in to see the labels
Use the scroll button to zoom in
and out.
If you don’t see the labels
Intermediate network graph
 crowded, overlapping labels and unpublishable.
Change label font size
Showing labels for only the significant compounds.
It is bit clearer.
Change node size
Select the values by press the left click
on mouse. Then right click.
Node size rules
FC 1.0 – size = 20
FC >1 & <2 --size = 60
FC >2 & < 3 -- size = 100
FC >3 & < 5 --size = 150
FC > 5-- size = 200
Intermediate network graph
Bit clearer, has experimental results. Highlighting the clusters that are changed.
 Not yet
publication ready
Node moving
Press “control” key and click left
mouse button and select the area
Now you can move
these nodes
Intermediate network graph
 Not yet
publication ready
Change edge colors
This box must be checked.
The visual property is
under the subtab – “edge”
Intermediate network graph
KEGG reactions
Chemical similarity
Lipids
Amino acids
and amines
Observations
• Several fatty acids and DAGs are increased in NAFLD
plasma.
• Metformin was higher in NAFLD subjects along with
increased in MTA and Hypoxanthine.
• PE, CER, PC and CEs were decreased in the NAFLD
subjects.
• Stachydrine- orange juice related compound was 5-
fold lower in the NFALD subjects.
• One carbon and lipid metabolism were altered in
the NAFLD subjects.
Cluster detection
Check this box
Large network can be divided into smaller modules for better
visualization and interpretation
Useful buttons in the menu-bar
Zoom in Zoom out Zoom-all
Zoom in
selected
You will use these often.
Clustered network
Create a sub-network
Select a cluster by pressing “Ctrl” and
then left click and make a square
box.
Once selected the nodes,
Prese Ctrl+N to make a new network
Show graphics
details
Node label position
Click on the label position
It will make label position property
available in the style tab.
Select right side nodes
Click on this box to
change the property
for selected node.
Drag the
object box
to the left
and click ok
Node label position
Increase the scaling factor to
remove the overlaps of labels.
Scaling
Focused view of the fatty acids and DG cluster.
Network navigation
Click on a network you want to visualize
Create
subnetworks for –
• Sphingolipids
• Cholesteroyl esters
• TGs
• Phopspholipids
• One carbon metabolism
Sphingolipid cluster
Cholestroyl esters
PC cluster + acetyl carnitines
Focused visualization of clusters
Clearer, readable, less crowded.
This can go in a paper. 
One carbon metabolism and FAFLD
The commonly used anti-diabetic agent metformin targets mitochondrial complex I and thus
decreases the NAD+/NADH ratio. Metformin also inhibits cancer cell growth, in part through
inhibition of biosynthetic metabolism (Griss et al., 2015). Metformin-induced growth
inhibition can be partially rescued by supplementation with hypoxanthine and thymidine,
products of 1C metabolism (Corominas-Faja et al., 2012). It remains unclear, however, if the
impact of metformin on 1C metabolism is clinically significant at normal therapeutic doses.
One carbon metabolism and FAFLD
Increased homocysteine also occurs in liver disease,
including non-alcoholic fatty liver disease (NAFLD) (Dai
et al., 2016). In animals fed high-fat diets to induce
NAFLD, liver 1C metabolism is dysregulated, as
evidenced by intrahepatic increases in SAH and free
homocysteine and decreases in methionine and the
GNMT enzyme (Pacana et al., 2015). At the same time,
deletions of 1C enzymes lead to development of liver
disease.
Save the session for future
Export the network as a pdf file
Conclusions
• Biochemical network created using KEGG or any
biochemical databases did not cover all the identified
metabolites.
• MetaMapp combined KEGG reactions and chemical
similarity mapping to put all the known metabolites into
biochemical modules
• Cytoscape provided rich functionalities to visualize and
cluster a network graphs.
• Overlaying statistical results on these graphs can highlight
the modules which were affected in cases in comparison
to controls.

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Metabolic network mapping for metabolomics

  • 1. Unit 5.2 & 5.5 Biochemical network mapping (MetaMapp) Dinesh Barupal dinkumar@ucdavis.edu
  • 2. DATA ACQUISITION Separation Detection SAMPLING EXTRACTION DATA PROCESSING File Conversion Baseline Correction Peak Detection Deconvolution Adduct Annotation Alignment Gap Filling STATISTICS Normalization Multivariate Analysis (Parametric, Nonparametric) Univariate Analysis (Unsupervised, Supervised) BIOLOGICAL INTERPRETATION Pathway Mapping Network Enrichment STUDY DESIGN VALIDATION COMPOUND IDENTIFICATION Molecular Formula ID Structure ID MS Library Search Database Search In silico Fragmentation WCMC UC Davis
  • 3. Questions : • Why a network graph ? • How to create biochemical network map of identified metabolites ? • How to include all the identified metabolites into a network ? • How to visualize and make publication ready network graphs ? • How to use MetaMapp and Cytoscape software ?
  • 4. What is a network graph ? A network graph represents entities as nodes (dots) and various relationships among them as edges (links). A C D B E relationship X An example network graph Nodes can be – genes, proteins, reactions, metabolites. Edges can be – correlation, reactions, reaction pairs, pathways, chemical similarity, mass spectral similarity. Edges can have direction like A B or B A. Notable examples – Air transportation network Citation/ co-author network Social network Metabolic network
  • 5. http://bmcgenomics.biomedcentral.com/articles/10.1186/1471-2164-13-334 What is a metabolic network ? Tools for make this type of network are – • MetScape (http://metscape.ncibi.org/) • MetaBox (www.metabox.fiehnlab.ucdavis.edu) • KEGG spider (https://genomebiology.biomedcentral .com/articles/10.1186/gb-2008-9-12- r179) • CPDB (http://consensuspathdb.org/) • MetExplore (http://metexplore.toulouse.inra.fr) A C D B E reaction X A metabolite Not every detected metabolite will be included in this network.
  • 6. Two representations of the EC 2.3.1.35 reaction. Two ways to convert a reaction to a graph The KEGG RPAIR database is a manually curated collection of reactant pairs (substrate-product pairs) and chemical structure transformation patterns in enzymatic reactions. Masanori Arita PNAS 2004;101:1543-1547 Connect only the actual subtract-product and ignore the side product or co-factors.
  • 7. Biochemical databases provide list of metabolites and reactions among them. An example of a metabolic reaction : http://www.brenda-enzymes.org/ http://www.genome.jp/kegg/ https://metacyc.org/ http://www.reactome.org/ Major DBs that provided curated list of biochemical reactions. Glucose- 6P D-Glucose D-Glucose 6-phosphate + H2O <=> D-Glucose + Orthophosphate http://www.genome.jp/dbget-bin/www_bget?rn:R00303 ~ 25000 metabolic reactions are known for various organisms. Node A Node B Node A Edge Node B Cpd 1 KEGG Cpd 2 Cpd 3 KEGG Cpd 4 Cpd 4 KEGG Cpd 5 Cpd 6 KEGG Cpd 7 … KEGG … Metabolic network in a text format How to make a metabolic network ? A C D B E reaction X A metabolite
  • 8. But not all the metabolites have reaction annotations ? https://bmcbioinformatics.biomedcentral.com/articl es/10.1186/1471-2105-13-99 https://www.nature.com/articles/s41598-017-15231-w Many significant (p<0.05) compounds are not present in pathway databases
  • 9. What is a chemical similarity coefficient ? A C D B E Chemical similarity A metabolite Xanthine Hypoxanthine Tanimoto Chemical Similarity score 0.917 Tanimoto = AB / ( A + B - AB ) Substructure decomposition for calculations of chemical similarity
  • 10. http://www.pnas.org/content/106/40/17187 What is a MetaMapp network ? All the identified metabolites are included in the graph.
  • 11. What is MetaMapp ? MetaMapp: mapping and visualizing metabolomic data by integrating information from biochemical pathways and chemical and mass spectral similarity https://bmcbioinformatics.biomedcentral.com/articles/10.1186/1471-2105-13-99 MetaMapp is a approach to map all the detected metabolites into a network graph that resembles known biochemistry Available at metamapp.fiehnlab.ucdavis.edu
  • 12. Input file : MetaMapp R- Package (openCPU version) Network file Node attribute file How to use MetaMapp ?
  • 13. How to get SMILES codes ?
  • 14. How to use MetaMapp ? Prepare the input file. • This is the minimum input • No duplicate CIDs are allowed Example : spring_2018_metabolomics_course_metamapp_ example.xlsx
  • 15. About the example dataset • Comparison of the plasma metabolome in Non alcoholic fatty liver disease subjects and the controls. • HILIC + CSH assays • ~ 650 identified metabolites. • Unpublished (you can write a paper out of it).
  • 16. MetaMapp input file errors - • Duplicate PubChem CIDs • Duplicate names • Missing SMILES codes • Missing p-value or fold-change • Headers mismatch • > 1000 compounds
  • 17. How to use MetaMapp ? Obtaining the MetaMapp files. • Go to http://metamapp.fiehnlab.ucdavis.edu Copy and paste your data in this box Click here Now, click on these two buttons chemsim_krp_07.sif node_attributes_chemsim_krp_07.tsv Both files are provided in the example folder for the case study.
  • 18. chemsim_krp_07.sif node_attributes_chemsim_krp_07.tsv Structure of the created files. Both files will be imported in the Cytoscape software for visualization KRP – KEGG Reaction Pairs – biochemical relationships TMSIM – Tanimoto similarity – chemical relationships
  • 19. What is Cytoscape ? The most used network visualization and analysis tool. http://journals.plos.org/plosbiology/article?id=10.1371%2Fjournal.pbio.1001843http://www.cytoscape.org/ Backed by strong institutions
  • 20. Visualize a range of experimental data on a network graph Useful graph layout algorithms Graph theory calculations Easy organization of multiple networks for comparisons. Faster navigation of large networks Filter and query the network Contributed plugins Works on PC, Max and Linux system USB drive contains a copy of Cytoscape software Cytoscape basic features
  • 21. Click here Start Cytoscape software Locate the chemsim_krp_07.sif file and click import. The file shall be in your download folder or you can use the file in the example folder. How to use Cytoscape?
  • 22. Import a new network If you want to import a new network file in already running Cytoscape Select the .sif file
  • 23. Visualization panel Table panel highlights the data related to selected node (yellow). Cytoscape windwos
  • 24. Show graphics details Tip: if you don’t see the labels/edges/shapes/colors in graph, click on “Show graphics details”.
  • 25. Visualize using the yFiles (organic layout). You can try other layout methods, but this one is recommended. Layout a network graph
  • 26. Network graph after organic layout
  • 27. Now import your Node Attributes file
  • 28. Import your Node Attributes file
  • 29. Import your Node Attributes file “Key” symbol should be PubChem_ID
  • 30. Import your Node Attributes file Table panel after importing the node attributes.
  • 31. Data visualization All visual properties can be accessed in the style tab. Node color Node size Node label Node label position Node Label font size Edge color Edge width Network background color
  • 32. Change network background color 1 2 3 Select black background color or any color you like.
  • 33. Double click here click here Node coloring : “Node Fill color”
  • 34. Red = higher Blue = lower Yellow = no change Node coloring : “Node Fill color”
  • 35. Change node label You can choose any label from the node attribute file. You need to zoom in to see the labels Use the scroll button to zoom in and out.
  • 36. If you don’t see the labels
  • 37. Intermediate network graph  crowded, overlapping labels and unpublishable.
  • 38. Change label font size Showing labels for only the significant compounds. It is bit clearer.
  • 39. Change node size Select the values by press the left click on mouse. Then right click. Node size rules FC 1.0 – size = 20 FC >1 & <2 --size = 60 FC >2 & < 3 -- size = 100 FC >3 & < 5 --size = 150 FC > 5-- size = 200
  • 40. Intermediate network graph Bit clearer, has experimental results. Highlighting the clusters that are changed.  Not yet publication ready
  • 41. Node moving Press “control” key and click left mouse button and select the area Now you can move these nodes
  • 42. Intermediate network graph  Not yet publication ready
  • 43. Change edge colors This box must be checked. The visual property is under the subtab – “edge”
  • 44. Intermediate network graph KEGG reactions Chemical similarity Lipids Amino acids and amines
  • 45. Observations • Several fatty acids and DAGs are increased in NAFLD plasma. • Metformin was higher in NAFLD subjects along with increased in MTA and Hypoxanthine. • PE, CER, PC and CEs were decreased in the NAFLD subjects. • Stachydrine- orange juice related compound was 5- fold lower in the NFALD subjects. • One carbon and lipid metabolism were altered in the NAFLD subjects.
  • 46. Cluster detection Check this box Large network can be divided into smaller modules for better visualization and interpretation
  • 47. Useful buttons in the menu-bar Zoom in Zoom out Zoom-all Zoom in selected You will use these often.
  • 49. Create a sub-network Select a cluster by pressing “Ctrl” and then left click and make a square box. Once selected the nodes, Prese Ctrl+N to make a new network Show graphics details
  • 50. Node label position Click on the label position It will make label position property available in the style tab.
  • 51. Select right side nodes Click on this box to change the property for selected node. Drag the object box to the left and click ok Node label position
  • 52. Increase the scaling factor to remove the overlaps of labels. Scaling Focused view of the fatty acids and DG cluster.
  • 53. Network navigation Click on a network you want to visualize Create subnetworks for – • Sphingolipids • Cholesteroyl esters • TGs • Phopspholipids • One carbon metabolism
  • 54. Sphingolipid cluster Cholestroyl esters PC cluster + acetyl carnitines Focused visualization of clusters Clearer, readable, less crowded. This can go in a paper. 
  • 56. The commonly used anti-diabetic agent metformin targets mitochondrial complex I and thus decreases the NAD+/NADH ratio. Metformin also inhibits cancer cell growth, in part through inhibition of biosynthetic metabolism (Griss et al., 2015). Metformin-induced growth inhibition can be partially rescued by supplementation with hypoxanthine and thymidine, products of 1C metabolism (Corominas-Faja et al., 2012). It remains unclear, however, if the impact of metformin on 1C metabolism is clinically significant at normal therapeutic doses. One carbon metabolism and FAFLD Increased homocysteine also occurs in liver disease, including non-alcoholic fatty liver disease (NAFLD) (Dai et al., 2016). In animals fed high-fat diets to induce NAFLD, liver 1C metabolism is dysregulated, as evidenced by intrahepatic increases in SAH and free homocysteine and decreases in methionine and the GNMT enzyme (Pacana et al., 2015). At the same time, deletions of 1C enzymes lead to development of liver disease.
  • 57. Save the session for future
  • 58. Export the network as a pdf file
  • 59. Conclusions • Biochemical network created using KEGG or any biochemical databases did not cover all the identified metabolites. • MetaMapp combined KEGG reactions and chemical similarity mapping to put all the known metabolites into biochemical modules • Cytoscape provided rich functionalities to visualize and cluster a network graphs. • Overlaying statistical results on these graphs can highlight the modules which were affected in cases in comparison to controls.

Notas do Editor

  1. Two representations of the EC 2.3.1.35 reaction. In this reaction, the acetyl moiety of N-acetyl l-ornithine is transferred to l-glutamate to form N-acetyl l-glutamate. (Lower Left) In the scheme of Jeong et al. (7), its two substrates and two products are equally linked to the object representing the EC number, irrespective of their structural changes. (Lower Right) In our scheme, conserved substructural moieties, coded by color, are computationally detected, and each link is associated with the information of which atom goes where.