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TN5 Transposase 3D Model

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TN5 Transposase royalty-free 3d model - Preview no. 1
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TN5 Transposase royalty-free 3d model - Preview no. 1
TN5 Transposase royalty-free 3d model - Preview no. 2
TN5 Transposase royalty-free 3d model - Preview no. 3
TN5 Transposase royalty-free 3d model - Preview no. 4
60
00
Royalty Free LicenseAll extended uses
Simple returns
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Works out of the box
487 visits
MichaelTaylor3D

Specifications

  • Geometrypolygonal
  • Polygons504,674
  • Vertices261,702
  • TexturesYes
  • RiggedNo
  • AnimatedNo
  • 3D Printable ReadyNo
  • Game Ready (low poly)No
  • UV MappedNo
  • Unwrapped UVsunknown

Formats & Files

3ds Max
(.max)
1 MB

TN5 TRANSPOSASE.zip
OBJ
(.obj)
7 MB

TN5 TRANSPOSASE obj.rar

Description

This is an scientifically accurate representation of an enzyme in High Definition. Enzymes are proteins that catalyze (i.e., increase the rates of) chemical reactions. In enzymatic reactions, the molecules at the beginning of the process are called substrates, and the enzyme converts them into different molecules, called the products. Almost all processes in a biological cell need enzymes to occur at significant rates. Since enzymes are selective for their substrates and speed up only a few reactions from among many possibilities, the set of enzymes made in a cell determines which metabolic pathways occur in that cell. Transposase Tn5 is a member of the RNase superfamily of proteins which includes retroviral integrases. Tn5 can be found in Shewanella and Escherichia bacteria. The transposon codes for antibiotic resistance to kanamycin and other aminoglycoside antibiotics. Tn5 and other transposases are notably inactive. Because DNA transposition events are inherently mutagenic, the low activity of transposases is necessary to reduce the risk of causing a fatal mutation in the host, and thus eliminating the transposable element. One of the reasons Tn5 is so unreactive is because the N- and C-termini are located in relatively close proximity to one another and tend to inhibit each other. This was elucidated by the characterization of several mutations which resulted in hyperactive forms of transposases. One such mutation, L372P, is a mutation of amino acid 372 in the Tn5 transposase. This amino acid is generally a leucine residue in the middle of an alpha helix. When this leucine is replaced with a proline residue the alpha helix is broken, introducing a conformational change to the C-Terminal domain, separating it from the N-Terminal domain enough to promote higher activity of the protein. The transposition of a transposon often needs only three pieces: the transposon, the transposase enzyme, and the target DNA for the insertion of the transposon.This is the case with Tn5, which uses a cut-and-paste mechanism for moving around transposons.
Jul 13, 2018 date added
Jan 24, 2022 last update

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