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生醫類器官 [Final Report]: Telencephalon Organoids D...

蔡秀吉
December 21, 2023

生醫類器官 [Final Report]: Telencephalon Organoids Derived from an Individual with ADHD Show Altered Neurodevelopment of Early Cortical Layer Structure

Source: Zhang, D., Eguchi, N., Okazaki, S. et al. Telencephalon Organoids Derived from an Individual with ADHD Show Altered Neurodevelopment of Early Cortical Layer Structure. Stem Cell Rev and Rep 19, 1482–1491 (2023). https://doi.org/10.1007/s12015-023-10519-z
I chose this very high-quality paper for my final report in school.

The reason I chose this paper is that brain organoids have been a very popular research topic in recent years. In addition, the reason for choosing psychiatric this kinda topic as my final report also bcuz I am now actually promoting this mental health leave at my school National Yang Ming chiao Tung University.

Other references:
* https://youtu.be/s5A1ysHGnp4(國立陽明交通大學神經工程實驗室
* 國家衛生研究院 全民健保研究資料庫(2017)
* https://pubmed.ncbi.nlm.nih.gov/12216060/

蔡秀吉

December 21, 2023
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  1. Telencephalon Organoids Derived from an Individual with ADHD Show Altered

    Neurodevelopment of Early Cortical Layer Structure Stem Cell Reviews and Reports Published online: 6 March 2023 https://doi.org/10.1007/s12015-023-10519-z Danmeng Zhang1, Noriomi Eguchi1, Satoshi Okazaki1, Ichiro Sora1, Akitoyo Hishimoto1
  2. Brain Development (Telencephalon) Embryonic brain regions Brain structures in child

    and adult Forebrain Midbrain Hindbrain Telencephalon Diencephalon Mesencephalon Metencephalon Myelencephalon Cerebrum (includes cerebral cortex, white matter, basal nuclei) Diencephalon (thalamus, hypothalamus, epithalamus) Midbrain (part of brainstem) Pons (part of brainstem), cerebellum Medulla oblongata (part of brainstem) Midbrain Forebrain Hindbrain Telencephalon Diencephalon Mesencephalon Metencephalon Myelencephalon Spinal cord Cerebrum Diencephalon Midbrain Pons Medulla oblongata Cerebellum Spinal cord Child Embryo at 5 weeks Embryo at 1 month
  3. Introduction to ADHD Characterized by Inattention, Hyperactivity, and Impulsivity. (Attention

    Deficit Hyperactivity Disorder) 注意力不足過動症 This disorder can cause failure in life activities such as Education and Communication throughout the lifetime.
  4. Pathophysiology ADHD is a neurodevelopmental disorder Prefrontal cortex (decision making,

    planning) Posterior Parietal Cortex (planned movements, spatial reasoning, and attention.) • (Timing) (Cognitive) Left-sided prefrontal cortex • Attention Distribution Posterior parietal cortex
  5. Amygdala Hippocampus ⚫ Amygdala 杏仁核 ⚫ Orbitofrontal cortex 框額葉 ⚫

    Hippocampus 海馬迴 ADHD compared with typical development (TD) Certain brain structure smaller in children with ADHD Orbitofrontal cortex
  6. Epidemiology of ADHD 台灣兒童&青少年(6~18歲) ~7.5% 約 20多萬 >5% 兒童青少年 >2.5%

    成年人 資料來源:國家衛生研究院 全民健保研究資料庫(2017) https://pubmed.ncbi.nlm.nih.gov/12216060/ ADHD is one of the most heritable neuropsychiatric disorders.
  7. The Rationale of use organoids Poor accessibility often makes it

    difficult to study them: postmortem brains of ADHD people are unavailable in many cases, and animal models cannot completely exhibit the phenotypes of ADHD. Brain organoids can mimic the early stage of neurodevelopment and pathology of neuropsychiatric disorders, suggesting that they have the potential to reveal the unknown mechanisms of ADHD. Organoids: The products of three-dimensional tissue culture using induced pluripotent stem cells (iPSCs), can recapitulate the development of human organs (including the brain) in vitro.
  8. Generation of Human iPSCs Donated by an 18-year-old male patient

    diagnosed with ADHD iPSCs of ADHD were generated from CD34-positive cells in mononuclear cells isolated from peripheral blood. • Pluripotency and Multipotency of iPSCs were confirmed by immunocytochemistry • Analyze chromosomes:No Abnormal Chromosomes in the iPSCs
  9. • From day 0 to day 18, the medium contained

    GMEM, 20% KSR, NEAA, 0.1 mM 2-ME, sodium pyruvate, IWR-1-endo and SB431542, human FGF2 (removed after day 6), and Y-27632 (added on day 3) • After day 18, the medium was changed to DMEM/F12 with GlutaMAX-I, N2 supplement, and chemically defined lipid concentrate, and floating cell aggregates were transferred to an EZSPHERE dish. • On day 35, 10% FBS, 5 mg/ml heparin, and 1% Matrigel (growth factor reduced) (Corning) were added to the medium (Supplementary Fig. 3). Cortical Tissues Differentiated from Human iPSCs Cortical differentiation from iPSCs using the modified SFEBq method Human iPSCs were dissociated into single cells and then reaggregated using cortical differentiation medium in 96-well V-bottom plates at a density of 5,000 cells per well. Half of the medium was changed every 3–4 days.
  10. Cortical Tissues Differentiated from Human iPSCs • After 35 or

    56 days of differentiation, the tissues were fixed in 4% PFA/PBS for 40 min and cryoprotected in 20% sucrose/PBS overnight at 4 °C. Fixed tissues were embedded in frozen section compound (Leica) and sliced into 10 µm thick sections. • The sliced tissues were transferred to CREST-coated glass slides (Matsunami Glass). Slides were washed with PBS, permeabilized with 0.3% Triton X-100 for 10 min, and blocked with 10% normal donkey serum in 0.3% Triton X-100/PBS for 30 min, followed by incubation with primary antibody overnight at 4℃. • Primary antibodies against the following antigens were used at the specified dilutions: FOXG1 (TakaRa, 1:1000), TUJ1 (Abcam, 1:1000), SOX2 (Abcam, 1:1000), CTIP2 (Abcam, 1:1000), TBR1 (Abcam, 1:1000; Santa Cruz), phospho-histone H3 (Cell Signaling, 1:500), cleaved caspase 3 (Cell Signaling, 1:200), and Ki67 (BD Pharmingen, 1:200). • Fluorescence-tagged secondary antibodies (Jackson) were reacted on the following day. The nuclei were counterstained with DAPI (BD Pharmingen, 1:2000).
  11. Results • Generation of Telencephalon Organoids • Thickness of Layer

    Structures in the Telencephalon Organoids • Thickness of CP and VZ • Number of Cells in Layer VI and V of the Cerebral Cortex • Number of Cell Divisions • Proportion of Symmetric and Asymmetric Cell Division • Apoptosis and Proliferation of Cells
  12. Generation of Telencephalon Organoids We used iPSCs from ADHD and

    control individuals to generate telencephalon organoids. After 35 days of differentiation (day 35), cell aggregates expressed FOXG1, a specific marker of the telencephalon (Fig. 1a). They contained cell layers expressing TUJ1 and SOX2, indicating layers of neurons and neural stem cells, similar to the cortical plate (CP) and ventricular zone (VZ) observed in the early neurodevelopment of the cerebral cortex (Fig. 1b). These results indicated that they successfully differentiated into telencephalon organoids and recapitulated the early cerebral cortex.
  13. • To distinguish morphological changes occurring in the early cortex

    in ADHD, we measured the thickness of layer structures in the telencephalon organoids (Fig. 1c). • Neuroepithelium-like structure (NE), defined as the total thickness of the CP and VZ, • Not significantly different between ADHD and control organoids on day 35. • The NE of ADHD-derived organoids was thinner than that of control-derived organoids on day 56. Thickness of Layer Structures in the Telencephalon Organoids
  14. • The thickness of the CP contained in the NE:

    • Significantly increased in both control and ADHD-derived organoids • ADHD-derived organoids was thinner than that of control-derived organoids on both day 35 and day 56. • The thickness of the VZ contained in the NE: • VZ was not significantly different between ADHD-derived and Control-derived on day 35. • ADHD-derived organoids was not significantly increased between day 35 and 56. • ADHD-derived was significantly thinner than Control-derived on day 56. In early development, ADHD organoids had a thinner (CP)cerebral cortex than Control organoids, may be due to the alteration in the VZ growth, the layer of neural stem cells. Comparison of CP and VZ thickness between day 35 and 56:
  15. • For further analysis of morphological differences, we counted the

    number of cells expressing TBR1 and/or CTIP2, specific marker proteins of neurons in layer VI and V of the cerebral cortex (Fig. 2a). • On day 35, the CP of ADHD organoids contained significantly more cells expressing CTIP2 and cells co- expressing TBR1 and CTIP2 than that of control organoids, even though their thickness was thinner than that of control organoids. • The number of cells expressing TBR1 and/or CTIP2 significantly increased between day 35 and 56 in control- derived organoids, whereas no significant increase was observed in ADHD-derived organoids. • These results showed altered growth of the early cortex, meaning that an increase in the number of neurons was disrupted in ADHD-derived organoids. Number of Cells in Layer VI and V of the Cerebral Cortex
  16. Number of Cell Divisions • Our morphological analysis showed that

    ADHD organoids had a thinner layer structure than control-derived, even though ADHD organoids have more neurons than control. • Suggested that alterations occurred in the neurodevelopment of ADHD organoids, including division of neural stem cells, differentiation from neural stem cells into neurons, and apoptosis of the cells. • For further investigation, we counted the number of cell divisions indicated by the expression of phospho-histone H3 (pHH3) (Fig. 3a). • In control-derived organoids, the number of cell divisions was not significantly changed between day 35 and 56 (Fig. 3b), indicating continuous proliferation of neural stem cells. Otherwise, in ADHD organoids, the number of cell divisions was significantly decreased from day 35 to 56, suggesting less potential to proliferate.
  17. Proportion of Symmetric and Asymmetric Cell Division Analyzed the proportion

    of symmetric and asymmetric cell division: cell division for the proliferation of neural stem cells and differentiation from neural stem cells into neurons. ⚫ When the angle between the plane of cell division and the apical surface was less than or equal to 30 degrees, the cell division was considered asymmetric division. ⚫ When the angle was greater than or equal to 60 degrees, the cell division was considered symmetric division (Fig. 3c).
  18. Proportion of Symmetric and Asymmetric Cell Division • From day

    35 to day 56, only the control organoids showed a significant change in the proportion of cell division (Fig. 3d), with an increase in asymmetric division and a decrease in symmetric division. • On day 56, the proportion of symmetric and asymmetric division showed a significant difference in control- and ADHD organoids: control-derived organoids showed more asymmetric division and less symmetric division than ADHD-derived organoids. • These results suggested that the proportion of cell division gradually shifted from proliferation to differentiation in a relatively later stage of development in control-derived organoids but not in ADHD-derived organoids.
  19. Apoptosis and Proliferation of Cells ⚫ Distinguished possible changes in

    cell death. We analyzed the amount of cleaved-caspase 3 (CC3) and Ki67, the marker protein for apoptosis and proliferation of cells (Fig. 4a). ⚫ In control-derived organoids, Ki67 was not significantly changed between day 35 and 56 (Fig. 4b), consistent with the pHH3 results. ⚫ On the other hand, in ADHD-derived organoids, proliferation significantly decreased between day 35 and 56. Cell death indicated by CC3 significantly decreased from day 35 to 56 in both control- and ADHD-derived organoids (Fig. 4c), although it was significantly higher in ADHD-derived organoids than in control-derived organoids on day 35. ⚫ These results indicated two characteristics of ADHD cells: the amount of cell proliferation was decreased in early development, and much apoptosis occurred. Alterations in proliferation and apoptosis might drive the changes in the morphology of layer structures and the number of neurons.
  20. Conclusions • Telencephalon organoids derived from ADHD patients exhibit altered

    neurodevelopment of the early cerebral cortex. • These findings suggest that alterations in neural stem cell proliferation, differentiation, and apoptosis may contribute to the pathogenesis of ADHD.