GMU:Life in an aquatic ecosystem/Dahye Seo

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Dead Life Live Life

Description

* This project was started but not completed in SS 2023 and will be continued this semester.

Dead Life Live Life is a sound installation work that sonifies the movement of DNA. This work was inspired by the poetic movement of DNA in electrophoresis experiments. Dead Life Live Life explores the materiality of DNA itself rather than genetic analysis, which is the general purpose of DNA. “Dead life got the same material as live life”, biologist Lynn Margulis said in an interview. This could be paraphrased as “Dead life got the same DNA as live life”. Dead Life Live Life poetically represents the connection between life and death by sonifying the DNA movement of an old persimmon tree planted in my grandmother's house.

Dlll 1.001.jpg
Dlll 2..jpg


Diagram Dead LifeLiveLife.jpg

Technical solution

1. Biological part

Instruction of DNA analysis

  • Instruction1 DNAworkshop.jpg
  • Instruction2 DNAworkshop.jpg

1) DNA Extraction of Persimmons

  • Kaki gelElectrophoresis 2.jpeg
  • Kaki gelElectrophoresis 3.jpeg
  • Kaki gelElectrophoresis 4.jpeg
  • Kaki gelElectrophoresis 5.jpeg
  • Kaki gelElectrophoresis 6.jpeg
  • Kaki gelElectrophoresis 7.jpeg
  • Kaki gelElectrophoresis 8.jpeg

2) PCR Experiment (DNA amplification) / Gel electrophoresis (DNA movement & visualization) .

  • Kaki gelElectrophoresis 10.jpeg
  • Kaki gelElectrophoresis 9.jpeg
  • Kaki gelElectrophoresis 11.jpeg
  • Kaki gelElectrophoresis 12.jpeg
  • Kaki gelElectrophoresis 13.jpeg
  • Gelelectrophoresis workshop 20230428 Large.jpeg

DNA of the persimmon is amplified through a PCR experiment. The amplified DNA is visualized in a gel electrophoresis experiment. DNA molecules dyed to respond to UV light glow and flow electromagnetically in an agar-gel chamber


2. Sound part

1) Sonification of DNA movementMax/Msp patch

Convert continuously changing number of RGB data (could be change to other data) of DNA movement animation to midi or frequency.

Load video
YouTube

2) Sound Design

Work in Biolab

2024.11.16. Sat, 9:30 am

Introduction

Gel Electrophoresis Exercise

I started by relearning how to use a micropipette to pick up where I left off a year ago. I tested two DNA ladders and a green stain that I had stored in the freezer to see if they were still functional.


Procedure

recipe

Agarosegel : 0.5g Agarose, 50 ml TBE Buffer, 2.5 µl DNA Stein green

TBE Buffer for cover gel : 50 ml TBE Buffer, 1.25 µl DNA Stein green

Gel Electrophoresis  : 5V - 40 min -> 5V - 40 min -> 6V - 60 min (current 400 in every process)

The instructions say to electrophoresis at 5v for 40 min. Due to the short distance of DNA migration, I did 2 additional cycles.

  • DNA ladder1.jpg
  • DNA Ladder2.jpg
  • Prepare GelElectrophoresis.jpg
  • Gel electrophoresis1.jpg
  • GelElectrophoresis.jpg
  • Note.jpg


Result

First Column: 1 kb DNA ladder

Last to first and second Columns: 100 bp DNA ladder

  • First round 5V-40min.jpg
  • 2round 5v-40min.jpg
  • 3round 6v-60min.jpg

*DNA moves slow. Next time, reduce the percentage of agarose gel ?

How to set up the current for the gel electrophoresis? Does it impact the value of current for the movement of DNA?

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Last modified
This page was last edited on 17 November 2024, at 11:43.