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Figure 3 • Purpose: To further characterize cell-to-cell transmission of αsynuclein using an in vitro coculture model • Figure 3(A) Hypothesis: If myc-tagged α-synuclein from donor cells can be released and transmitted to SH-SY5Y acceptor cells, then αsynuclein will be detected in the donor cells via immunofluorescence. Figure 3 SH-SY5Y myc myc myc myc myc SH-SY5Y + α-synuclein Donor Cells Q Q Q Q Q SH-SY5Y Acceptor Cells Figure 3(A): Results • After 24 hrs, myc-tagged α-synuclein from donor cells was detected in acceptor cells • Formation of inclusion bodies in some acceptors cells Figure 3(A): Results • After 24 hrs, myc-tagged α-synuclein from donor cells was detected in acceptor cells • Formation of inclusion bodies in some acceptors cells *, p<0.05 **, p< 0.01 Conclusions? Figure 3(B): Results • Inclusion body formation occurs with prolonged transmission of α-synuclein Conclusions? Figure 3(C) • ~ ½ of the acceptor cells displayed ubiquitin immunoreactivity Figure 3(D) • Cell-to-cell transmission occurs without cellular membrane leakage Conclusions? Supplemental Fig. S3A • Purpose: To determine if transmission of α-synuclein aggregates is dependent on endocytosis – Dynamin-1 K44A expressed in acceptor cells (blocks endocytic formation) – Donor cells cocultured with acceptor cells • Hypothesis: If transmission of α-synuclein aggregates is dependent on endocytosis, then we would detect a reduction in the uptake of α-synuclein in the cells expressing dynamin-1 K44A. Fig. S3A: Results • Transmission of α-synuclein significantly reduced in acceptor cells **, p< 0.01 Conclusions? Figure 4 • Increased α-synuclein accumulation by lysosomal failure but no effect on proteosomal inhibition Conclusions? Figure 5 • Purpose: To examine the toxicity of endocytosed neuron-derived extracellular α-synuclein to the neurons • Hypothesis: If secreted/endocytosed α-synuclein is toxic to the cells, then we would expect to detect neuronal degeneration and caspase 3 activation. Figure 5 (A & B): Results • Neurons showed nuclear fragmentation and increased immunoreactivity of activated caspase 3 over 3 days *, p<0.05 **, p< 0.01 Figure 5 (C): Results • MCNSCs showed activated caspase 3 immunoreactivity within 4 weeks *, p<0.05 Conclusions? Overall Conclusions 1. There is evidence for direct cell-to-cell transmission of αsynuclein. 2. Nerve cells that overexpress tagged α-synuclein can transmit the protein to neural stem cells both in vivo and in vitro. 3. Inclusion body formation occurs with prolonged transmission of α-synuclein. 4. α-synuclein accumulation is achieved when protein quality control systems of the acceptor cells are inhibited. 5. Acceptor neuronal stem cells exhibit cell death and activated caspase 3 due to α-synuclein propagation. So, why do we care? • Is Parkinson’s Disease really a problem of protein aggregation? • PD is characterized by neuron death and the surviving neurons show aggregations of α-synuclein • If α-synuclein aggregates into an insoluble Lewy Body, PD develops So, why do we care? • Deposition of Lewy-like inclusions from host to grafted neurons in human PD patients is age-dependent • Understanding how to control α-synuclein aggregation in & around neurons could lead to revolutionary treatment of Parkinson’s Disease • How can we treat PD (based on Desplats et al.’s paper?)
