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Major seminar
Organ on a chip- Replacement of laboratory
animals
Submitted by
Ranjitha H.B.
P-2082 (IVRI)
Division of Veterinary Biotechnology
Contents
• Drug development model
• Organ on a chip
• Microfluidics
• Fabrication method
• Lung on a chip
• Human disease model
• Eye on a chip
• Gut on a chip
• Kidney glomerulus on a chip
• Liver on a chip
• Conclusion
The big challenge: Current drug
development model
Why the drug development model is broken
• Cost to develop and approve a new drug >$2.5
billion
• Cells cultured in dishes don’t function like in our
bodies
• Animal studies takes years to complete
• Innumerable animal lives are lost
• Results often don’t predict clinical response
Need better lab models that mimic
whole human organ function
ORGAN-ON-A-CHIP
Human cells
Structure
Environment
• Microengineered biomimetic system
• Engineer microchips containing living
human cells that reconstitute organ-level
functions
Uses:
-to test efficacy, toxicity of drugs and chemicals
-to create in vitro models of human disease
Microfluidics
• Science of manipulating small amounts (10–9 to 10–18 L) of
fluids in microfabricated hollow channels
• Advantages-
-It offers control of features at same size scale of living cells
-Tune dynamic fluid flows and spatiotemporal gradients
-Sample saving
Whitesides, G.M. 2006
Fabrication methods for microfluidic chips
Huh et al., 2011; Bhatiya et al., 2014
a) Photolithography
b)Microfluidic devices- PDMS substrate containing microchannel features
created by replica molding with a blank PDMS slab.
b) Soft lithography
Lung on a chip
Patton & Byron, Nat. Rev. drug discovery
AIR
BLOOD
BIODESIGN PRINCIPLES:
• Tissue-Tissue interface
• Dynamic flow
• Cyclic breathing movements
Huh et al., 2010
Design of lung on a chip
From design to device
Huh et al., 2013 Nature protocol
Human disease model:
Pulmonary edema in a lung-on-a-chip
Huh et al., 2012. Sci. Trans. Med.
Clinically relevant dose of IL-2 (1000 U/ml)
Effects of IL-2 cancer drug on lung permeability
depends on mechanical breathing motions
On chip
Vascular
leakage
model
Prediction
confirmed
In Vivo
Discovery of mechanotherapeutic
Huh et al., 2012
Eye on a chip
(A) Porous polystyrene shell scaffolds (5mm) (B)Scanning electron microscope (SEM) images of the scaffolds, 500 μm and 50 μm
(inset). (C) Formation of corneal stroma on scaffold pores with keratocytes and type I collagen gel (D)Confocal image of fluorescently
labeled keratocytes. Green and blue represent cytoplasmic and nuclear staining,espectively. (E) 3D patterning of green and red
HCECs on the curved scaffold surface to recapitulate human corneal and conjunctival tissues.
Seo & Huh, 2014
Gut on a chip
Microbial co-culture on a human intestinal epithelial monolayer
Kim et al., 2012
Gut-on-a-chip device Phase-contrast micrograph of intestinal vili
Cellbarrier
Human kidney proximal tubule-on-a-chip
(nephrotoxicity assessment)
Design for the human kidney proximal tubule-on-a-chip
Cell morphology
under static conditions
versus flowAnalysis of proximal tubular epithelial cell functions
Jang et al., 2013
Cisplatin toxicity measured in vitro
Apoptosis, as determined by TUNEL assay
Immunofluorescence views of Annexin V
Jang et al., 2013
Kidney glomerulus on a chip
Organ chip lined by-
•Human iPS derived kidney podocytes
•Human glomerular microvascular endothelium
Musah et al., 2017
Liver on a chip
Microfluidic liver sinusoid
Hepatotoxicity of diclofenac on human hepatocytes. The
drug was prepared at 100–700 mM in cell culture medium
and exposed to human hepatocytes in the microfluidic
sinusoid for 4 h ( ) and 24 h ( ).
Lee et al., 2007
Liver on a chip response to
acetaminophen, N-acetyl-L-cysteine
countermeasure
Viability as determined by LIVE/DEAD staining
Green – Calcein AM-stained viable cells; Red –
Ethidium homodimer-stained dead cells
Skardal et al., 2017
Soohee Cho & Jeong-Yeol Yoon, 2017
Advantages
• Replace animal models
• Study on interactions of pathogens & organ
cells, mechanism of virus infection
• To study effect of drug on target organ and
also others
• Study of toxicity of drugs and cosmetics
• To study cancer cells and produce new drugs
• Helps in pharmacological studies
Disadvantages of organ on a chip
• Some organ functions—cognition in the brain,
mechanical function in bone, ligaments, tendons
cannot be readily modeled on chips
• Specialized microengineering capabilities
• microbial contamination
• Chronic disease???
Huh, along with Donald Ingber of Harvard’s Wyss Institute,
received the Design Museum of London’s 2015 Design of the
Year award
Conclusion
The potential for transformative change-
As an alternative to conventional cell culture &
animal models, human organs-on-chips could
transform many areas of basic research and drug
development. They could be applied to research on
molecular mechanisms of organ development, disease
& on the interactions of the body with stimuli such as
drugs, environmental agents, consumer products and
medical devices.
•Thank you
• References
• Whitesides, G.M., 2006. The origins and the future of
microfluidics. Nature, 442(7101): 368.
• Huh, D., Hamilton, G.A. and Ingber, D.E., 2011. From 3D cell culture to organs-on-
chips. Trends in cell biology, 21(12): 745-754.
• Huh, D., Kim, H.J., Fraser, J.P., Shea, D.E., Khan, M., Bahinski, A., Hamilton, G.A.
and Ingber, D.E., 2013. Microfabrication of human organs-on-chips. Nature
protocols, 8(11): 2135.
• Esch, E.W., Bahinski, A. and Huh, D., 2015. Organs-on-chips at the frontiers of
drug discovery. Nature reviews. Drug discovery: 248.
• Bhatia, S.N. and Ingber, D.E., 2014. Microfluidic organs-on-chips. Nature
biotechnology: 760-772.
• Sung, J.H., Esch, M.B., Prot, J.M., Long, C.J., Smith, A., Hickman, J.J. and Shuler,
M.L., 2013. Microfabricated mammalian organ systems and their integration into
models of whole animals and humans. Lab on a Chip, 13(7): 1201-1212.
• Huh, D., Leslie, D.C., Matthews, B.D., Fraser, J.P., Jurek, S., Hamilton, G.A.,
Thorneloe, K.S., McAlexander, M.A. and Ingber, D.E., 2012. A human disease
model of drug toxicity–induced pulmonary edema in a lung-on-a-chip
microdevice. Science translational medicine, 4(159): 159ra147-159ra147.

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Organ on a chip- replacement of laboratory animal

  • 1. Major seminar Organ on a chip- Replacement of laboratory animals Submitted by Ranjitha H.B. P-2082 (IVRI) Division of Veterinary Biotechnology
  • 2. Contents • Drug development model • Organ on a chip • Microfluidics • Fabrication method • Lung on a chip • Human disease model • Eye on a chip • Gut on a chip • Kidney glomerulus on a chip • Liver on a chip • Conclusion
  • 3. The big challenge: Current drug development model
  • 4. Why the drug development model is broken • Cost to develop and approve a new drug >$2.5 billion • Cells cultured in dishes don’t function like in our bodies • Animal studies takes years to complete • Innumerable animal lives are lost • Results often don’t predict clinical response Need better lab models that mimic whole human organ function
  • 5. ORGAN-ON-A-CHIP Human cells Structure Environment • Microengineered biomimetic system • Engineer microchips containing living human cells that reconstitute organ-level functions Uses: -to test efficacy, toxicity of drugs and chemicals -to create in vitro models of human disease
  • 6. Microfluidics • Science of manipulating small amounts (10–9 to 10–18 L) of fluids in microfabricated hollow channels • Advantages- -It offers control of features at same size scale of living cells -Tune dynamic fluid flows and spatiotemporal gradients -Sample saving Whitesides, G.M. 2006
  • 7. Fabrication methods for microfluidic chips Huh et al., 2011; Bhatiya et al., 2014 a) Photolithography b)Microfluidic devices- PDMS substrate containing microchannel features created by replica molding with a blank PDMS slab. b) Soft lithography
  • 8. Lung on a chip Patton & Byron, Nat. Rev. drug discovery AIR BLOOD BIODESIGN PRINCIPLES: • Tissue-Tissue interface • Dynamic flow • Cyclic breathing movements Huh et al., 2010
  • 9. Design of lung on a chip
  • 10. From design to device Huh et al., 2013 Nature protocol
  • 11. Human disease model: Pulmonary edema in a lung-on-a-chip Huh et al., 2012. Sci. Trans. Med. Clinically relevant dose of IL-2 (1000 U/ml)
  • 12. Effects of IL-2 cancer drug on lung permeability depends on mechanical breathing motions On chip Vascular leakage model Prediction confirmed In Vivo Discovery of mechanotherapeutic Huh et al., 2012
  • 13. Eye on a chip (A) Porous polystyrene shell scaffolds (5mm) (B)Scanning electron microscope (SEM) images of the scaffolds, 500 μm and 50 μm (inset). (C) Formation of corneal stroma on scaffold pores with keratocytes and type I collagen gel (D)Confocal image of fluorescently labeled keratocytes. Green and blue represent cytoplasmic and nuclear staining,espectively. (E) 3D patterning of green and red HCECs on the curved scaffold surface to recapitulate human corneal and conjunctival tissues. Seo & Huh, 2014
  • 14. Gut on a chip Microbial co-culture on a human intestinal epithelial monolayer Kim et al., 2012 Gut-on-a-chip device Phase-contrast micrograph of intestinal vili Cellbarrier
  • 15. Human kidney proximal tubule-on-a-chip (nephrotoxicity assessment) Design for the human kidney proximal tubule-on-a-chip Cell morphology under static conditions versus flowAnalysis of proximal tubular epithelial cell functions Jang et al., 2013
  • 16. Cisplatin toxicity measured in vitro Apoptosis, as determined by TUNEL assay Immunofluorescence views of Annexin V Jang et al., 2013
  • 17. Kidney glomerulus on a chip Organ chip lined by- •Human iPS derived kidney podocytes •Human glomerular microvascular endothelium Musah et al., 2017
  • 18. Liver on a chip Microfluidic liver sinusoid Hepatotoxicity of diclofenac on human hepatocytes. The drug was prepared at 100–700 mM in cell culture medium and exposed to human hepatocytes in the microfluidic sinusoid for 4 h ( ) and 24 h ( ). Lee et al., 2007
  • 19. Liver on a chip response to acetaminophen, N-acetyl-L-cysteine countermeasure Viability as determined by LIVE/DEAD staining Green – Calcein AM-stained viable cells; Red – Ethidium homodimer-stained dead cells Skardal et al., 2017
  • 20. Soohee Cho & Jeong-Yeol Yoon, 2017
  • 21. Advantages • Replace animal models • Study on interactions of pathogens & organ cells, mechanism of virus infection • To study effect of drug on target organ and also others • Study of toxicity of drugs and cosmetics • To study cancer cells and produce new drugs • Helps in pharmacological studies
  • 22. Disadvantages of organ on a chip • Some organ functions—cognition in the brain, mechanical function in bone, ligaments, tendons cannot be readily modeled on chips • Specialized microengineering capabilities • microbial contamination • Chronic disease???
  • 23. Huh, along with Donald Ingber of Harvard’s Wyss Institute, received the Design Museum of London’s 2015 Design of the Year award
  • 24. Conclusion The potential for transformative change- As an alternative to conventional cell culture & animal models, human organs-on-chips could transform many areas of basic research and drug development. They could be applied to research on molecular mechanisms of organ development, disease & on the interactions of the body with stimuli such as drugs, environmental agents, consumer products and medical devices.
  • 26. • References • Whitesides, G.M., 2006. The origins and the future of microfluidics. Nature, 442(7101): 368. • Huh, D., Hamilton, G.A. and Ingber, D.E., 2011. From 3D cell culture to organs-on- chips. Trends in cell biology, 21(12): 745-754. • Huh, D., Kim, H.J., Fraser, J.P., Shea, D.E., Khan, M., Bahinski, A., Hamilton, G.A. and Ingber, D.E., 2013. Microfabrication of human organs-on-chips. Nature protocols, 8(11): 2135. • Esch, E.W., Bahinski, A. and Huh, D., 2015. Organs-on-chips at the frontiers of drug discovery. Nature reviews. Drug discovery: 248. • Bhatia, S.N. and Ingber, D.E., 2014. Microfluidic organs-on-chips. Nature biotechnology: 760-772. • Sung, J.H., Esch, M.B., Prot, J.M., Long, C.J., Smith, A., Hickman, J.J. and Shuler, M.L., 2013. Microfabricated mammalian organ systems and their integration into models of whole animals and humans. Lab on a Chip, 13(7): 1201-1212. • Huh, D., Leslie, D.C., Matthews, B.D., Fraser, J.P., Jurek, S., Hamilton, G.A., Thorneloe, K.S., McAlexander, M.A. and Ingber, D.E., 2012. A human disease model of drug toxicity–induced pulmonary edema in a lung-on-a-chip microdevice. Science translational medicine, 4(159): 159ra147-159ra147.

Editor's Notes

  1. Accelerate drug development and replace animal testing
  2. Huh et al., 2011
  3. Softlithography
  4. Huh et al., 2010
  5. recapitulated organ-level physiological functions, including pulmonary vascular barrier integrity and inflammatory responses to pathogens,
  6. widths of the central cell culture channel and two side vacuum channels are 400 µm and 200 µm, respectively
  7. establishing a human lung disease model on-chip that reconstitutes these toxic side effects of IL-2 and resultant pulmonary edema in patients. We also investigated the possibility that mechanical breathing motions might contribute to pulmonary toxicity of IL-2 and tested whether therapeutics such as angiopoietin-1 (Ang-1) and a new inhibitor of transient receptor potential vanilloid 4 (TRPV4), GSK2193874 (GlaxoSmithKline), can suppress pulmonary vascular leakage in this in vitro human disease model, and hence have the potential to treat human patients.
  8. Discovery of a mechanotherapeutic
  9. we first plated human corneal epithelial cells (HCECs) labeled with a green fluorescent dye at the center of the scaffold surface, and this step was followed by seeding of red-stained HCECs at the peripheral region. Simulation of eye blinking was accomplished by integrating a 3D-printed biomimetic eyelid into the upper chamber of the device. Blinking patterns and kinematics such as velocity, durations, and frequencies were precisely controlled by a computerized miniature DC motor.
  10. Cell barrier
  11. cisplatin (100 mM)
  12. Organ chip lined by- Human iPS derived kidney podocytes Human glomerular microvascular endothelium, The proximal tubule is of particular interest for studies on nephrotoxicity because active clearance, reabsorption, intracellular concentration, and local interstitial accumulation of drugs occur primarily at this site in the kidney
  13. Primary hepatocytes represent a physiologically relevant model for drug toxicity screening imilar to a human liver sinusoid, each unit consisted of 250 tightly packed hepatocyte s receiving nutrient flow of approximately 100 pL/s. chip was designed to handle eight individual inlet/outlet conditions, with each unit consisting of four parallel microfluidic sinusoids, 4 h ( *) and 24 h (&).
  14. Skardal et al., 2017
  15. Adv: high-resolution imaging ability to control fluid flow Inclusion of flow
  16. which enhances the differentiation, function and long-term survival of many cell types, allows testing of microenvironmental chemical signals, such as chemical, oxygen and cytokine gradients, as well as hormonal (soluble signals between organs) and angiocrine (soluble signals from endothelium) cues.