Difference between revisions of "Part:BBa K3113050"

 
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<h2>Usage and Biology</h2>
 
<h2>Usage and Biology</h2>
  
The CD63-including superfamily of tetraspanins are cell surface-associated membrane proteins, composed of four alpha-helical transmembrane domains with two extracellular loops.CD63 was the first characterized tetraspanin. It is abundantly represented in late endosomes and lysosomes as well as exosomes. The gene, coding for CD63, is located on the human chromosome 12q13. Although the intracellular function of CD63 remains to be established, a number of studies performed in different cell types implicate a role for CD63 in intracellular transport of other proteins.<ref>Trafficking and function of the tetraspanin CD63
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The CD63-including superfamily of tetraspanins are cell surface-associated membrane proteins, composed of four alpha-helical transmembrane domains with two extracellular loops. CD63 was the first characterized tetraspanin. It is abundantly represented in late endosomes and lysosomes, as well as exosomes. The gene, coding for CD63, is located on the human chromosome 12q13. Although the intracellular function of CD63 remains to be elucidated, a number of studies performed in different cell types implicate a role for CD63 in intracellular transport of other proteins.<ref>Trafficking and function of the tetraspanin CD63
 
Cell Microscopy Center, Department of Cell Biology and Institute of Biomembranes, University Medical Center Utrecht, Heidelberglaan 100, 3584CX Utrecht, The Netherlands
 
Cell Microscopy Center, Department of Cell Biology and Institute of Biomembranes, University Medical Center Utrecht, Heidelberglaan 100, 3584CX Utrecht, The Netherlands
 
Received 16 September 2008, Accepted 23 September 2008, Available online 7 October 2008.</ref>
 
Received 16 September 2008, Accepted 23 September 2008, Available online 7 October 2008.</ref>
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<h3>HiBiT Export</h3>
 
<h3>HiBiT Export</h3>
  
We can successfully secrete CD63-containing exosomes from HEK293T cells 48h after transfection as shown in Figure 1. As observed on the image below, exosomes containing the adapter L7Ae are expressed in approximatelly 150 pmol HiBiT-equivalents. Most importantly, the secretion efficiency of loaded exosomes is notably higher compared to control samples lacking the engineered CD63-construct and even twice as high as the secretion efficiency of empty exosomes lacking the RNA-binding protein (RBP).
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We can successfully secrete CD63-containing exosomes from HEK293T cells 48h after transfection as shown in Fig. 1B. Engineered exosomes containing the adapter L7Ae were expressed in approximatelly 150 pmol HiBiT-equivalents (Fig. 1B). Gag VLPs containing L7Ae adapter show expression in approximatelly 35 pmol HiBiT equivalents (Fig. 1A). Most importantly, the secretion efficiency of loaded exosomes is notably higher compared to control samples lacking the engineered CD63-construct and even twice as high as the secretion efficiency of empty exosomes lacking the RNA-binding protein (RBP).
  
 
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<figure class="figure">
 
<figure class="figure">
                 <img src="" width="400" height="360" class="figure-img img-fluid rounded" alt="Secretion efficiency of exosome vesicles calculated from HiBiT-measurements.">
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                 <img src="https://2019.igem.org/wiki/images/e/ec/T--Munich--Secretionefficiency_2.png" width="75%" class="figure-img img-fluid rounded" alt="Secretion efficiency of exosome vesicles calculated from HiBiT-measurements.">
 
                     <figcaption class="figure-caption"><b>
 
                     <figcaption class="figure-caption"><b>
Figure 1: Secretion efficiency of exosomes calculated from HiBiT-measurements.</b> Loaded vesicles containing the adapter L7Ae as well as empty exosomes lacking the RNA binding protein (RBP) were secreted from HEK293T cells with efficiencies of more than 100 pmol of HiBiT-equivalent. In contrast, control samples transfected with mock DNA did not show any secretion. Measurements were performed for n = 6 biological replicates in a 96-well format.  
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Figure 1: Secretion efficiency of VLPs (A) and exosomes (B) calculated from HiBiT-measurements.</b> Loaded vesicles containing the adapter L7Ae as well as empty exosomes lacking the RNA binding protein (RBP) were secreted from HEK293T cells with efficiencies of more than 100 pmol HiBiT-equivalents. In contrast, lower expression is observed in case of VLPs. Control samples transfected with mock DNA did not show any secretion. Measurements were performed for n = 6 biological replicates in a 96-well format.  
  
 
                     </figcaption>
 
                     </figcaption>

Latest revision as of 01:41, 22 October 2019


CD63

CD63 is a protein that belongs to the family of tetraspanins. It is a cell surface receptor for Timp-1 and plays a role in the activation of cellular signaling cascades. CD63 can be used to load RNA or proteins into extracellular vesicles.


Usage and Biology

The CD63-including superfamily of tetraspanins are cell surface-associated membrane proteins, composed of four alpha-helical transmembrane domains with two extracellular loops. CD63 was the first characterized tetraspanin. It is abundantly represented in late endosomes and lysosomes, as well as exosomes. The gene, coding for CD63, is located on the human chromosome 12q13. Although the intracellular function of CD63 remains to be elucidated, a number of studies performed in different cell types implicate a role for CD63 in intracellular transport of other proteins.[1]

Characterization

HiBiT Export

We can successfully secrete CD63-containing exosomes from HEK293T cells 48h after transfection as shown in Fig. 1B. Engineered exosomes containing the adapter L7Ae were expressed in approximatelly 150 pmol HiBiT-equivalents (Fig. 1B). Gag VLPs containing L7Ae adapter show expression in approximatelly 35 pmol HiBiT equivalents (Fig. 1A). Most importantly, the secretion efficiency of loaded exosomes is notably higher compared to control samples lacking the engineered CD63-construct and even twice as high as the secretion efficiency of empty exosomes lacking the RNA-binding protein (RBP).

Secretion efficiency of exosome vesicles calculated from HiBiT-measurements.
Figure 1: Secretion efficiency of VLPs (A) and exosomes (B) calculated from HiBiT-measurements. Loaded vesicles containing the adapter L7Ae as well as empty exosomes lacking the RNA binding protein (RBP) were secreted from HEK293T cells with efficiencies of more than 100 pmol HiBiT-equivalents. In contrast, lower expression is observed in case of VLPs. Control samples transfected with mock DNA did not show any secretion. Measurements were performed for n = 6 biological replicates in a 96-well format.


Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    COMPATIBLE WITH RFC[25]
  • 1000
    COMPATIBLE WITH RFC[1000]

References

  1. Trafficking and function of the tetraspanin CD63 Cell Microscopy Center, Department of Cell Biology and Institute of Biomembranes, University Medical Center Utrecht, Heidelberglaan 100, 3584CX Utrecht, The Netherlands Received 16 September 2008, Accepted 23 September 2008, Available online 7 October 2008.