Difference between revisions of "Part:BBa K5184032"

Latest revision as of 12:18, 2 October 2024

Cs1A

In order to eliminate spider mites, spider venom peptide Cs1A is incorporated in our project to broaden the spectrum of molecular targets of venom peptides. Cs1a is a small cysteine-rich venom peptide derived from Calommmata signata. Utilized as predatory toxin in nature, it carries the ability to cause paralysis and death in susceptible subjects by interfering with voltage-gated calcium channels. Given CaV channels' roles in neurotransmitter release and neural impulse relay, Cs1A serves as an effective pesticide.

Sequences

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]

Usage and Biology

Cs1A is a 32aa long peptide containing 6 cysteine residues arranged to create a cysteine framework of C1xxxC2xxxC3C4xxxC5xxxC6, forming cysteine cross bridges between C1C3, or C1C4, and between C2C5 or C2C6 [Fig1A].

Fig1: (A) Cysteine cross-bridge structure in Cs1A B. Secondary structure of Cs1A, by structural prediction results from AlphaFold. The cyestine residues are colored orange, displaying their side chains and the rest of the peptide in white

Paralysis and mortal effects of susceptible subjects are achieved via Cs1A inhibition on both high-voltage-activated (HVA) Cav channels and low-voltage-activated (LVA) Cav channels of susceptible targets by blocking the channels directly, resulting in impediment of fundamental nervous system responses in neuronal, muscular, and cardiac functions. (Specific site of inhibition depends on the concentration of neurotoxin).

Toxicity Verification

Cs1A is synthesized using the vector pET28a-G1M5-His-SUMO-Cs1A-GNA-His[Fig2B], of which is assembled using GoldenGate cloning and transformed into E. coli strain DH5ɑ. Colony PCR and sequencing is then carried out to verify the plasmid construct, of which is extracted and transformed into BL21(DE3) strain for expression. After IPTG induction and overnight incubation, the liquid culture is harvested and, after cell lysis, have an SDS-PAGE run. The results suggest that Cs1A had achieved soluble expression. After several unsuccessful purification attempts, the supernatant is treated directly by SUMO protease [Fig2C].

Fig2: (A) G1M5 tag allows secretion of the fusion protein into extracellular milieu (B) Plasmid construct pET28a-G1M5-His-SUMO-Cs1A-GNA-His (C) SDS-PAGE of supernatant and SUMO-treated supernatant, with supernatant of similarly treated supernatant of BL21(DE3) as control

The SUMO-digested supernatant's toxicity against T. urticae females is tested using a spraying method by Professor Huang from SCAU. Results from the toxicity assay suggests Cs1A to be highly toxic against T. urticae, achieving an fatality of 92.73% within 72 hours.

Fig3: (A) T. urticae in their normal state, before being sprayed with treated supernatant (B) Dead T. urticae from spraying of treated supernatant (C) Survival plot of T. urticae being sprayed with supernatant containing Cs1A over 72 hours, CK is similarly processed supernatant of BL21(DE3), acting as a control (D) Lethality data of T. urticae being sprayed with supernatant over 24, 48, and 72 hours, CK is the similarly processed supernatant of BL21(DE3), acting as a control

Part Collection

Our part collection provides a comprehensive list of venom peptides with a diverse range of molecular targets, and all displays satisfactory elimination efficacy during our testings [Fig7A&B].

Fig7: A. Survival plot of 6 venom peptides against female T. urticae using a spraying method, CK is induced liquid culture of BL21(DE3), of which acts as control D. Lethality data of 6 venom peptides over 24, 48, and 72 hours, CK is induced liquid culture of BL21(DE3), of which acts as control; data is the means of ± SD of three parallel replicate experiments

Our Part Collection
Current VP	Venom Name	Targeted Ion Channel	New?	Part Number	Original Specie
	PpVP2S	Ca	New	BBa_K5184043	Phytoseiulus persimilis
	PpVP1S	Ca	New	BBa_K5184042	Phytoseiulus persimilis
	PpVP1F	Ca	New	BBa_K5184038	Phytoseiulus persimilis
	rCtx4	Na		BBa_K5184021	Phoneutria depilata
✳️	Cs1A	Ca		BBa_K5184032	Calommata signata
	HxTx-Hv1h	Ca, K		BBa_K5184033	Hadronyche versuta

@@ Line 3: / Line 3: @@
 <partinfo>BBa_K5184032 short</partinfo>
-Cs1a is a small cysteine-rich venom peptide derived from Calommmata signata. In nature, utilized as predatory toxin, it carries the ability to cause paralysis and death in susceptible subjects by blocking voltage-gated calcium channels of susceptible targets. Having the voltage-gated calcium channels playing a fundamental role in neuronal, muscular and cardiac functions, targets experience fast immobilization after envenomation. In the context of our project, Cs1A is utilized as a sustainable pesticide to eliminate spider mites on infectious cultivations by targeting their ion channels. It is expressed via Escherichia. Coli strand OrigamiB and injected into crickets to test mortal effects.
+In order to eliminate spider mites, spider venom peptide Cs1A is incorporated in our project to broaden the spectrum of molecular targets of venom peptides. Cs1a is a small cysteine-rich venom peptide derived from ''Calommmata signata''. Utilized as predatory toxin in nature, it carries the ability to cause paralysis and death in susceptible subjects by interfering with voltage-gated calcium channels. Given CaV channels' roles in neurotransmitter release and neural impulse relay, Cs1A serves as an effective pesticide.
-<!-- Add more about the biology of this part here
-===Usage and Biology===
+===Sequences===
 <!-- -->
 <span class='h3bb'>Sequence and Features</span>
 <partinfo>BBa_K5184032 SequenceAndFeatures</partinfo>
+===Usage and Biology===
+Cs1A is a 32aa long peptide containing 6 cysteine residues arranged to create a cysteine framework of C1xxxC2xxxC3C4xxxC5xxxC6, forming cysteine cross bridges between C1C3, or C1C4, and between C2C5 or C2C6 [Fig1A].
+<center><html><img src="https://static.igem.wiki/teams/5184/parts/cs1a-structure.webp" width="600"/></html></center>
+<center><b>Fig1: (A) Cysteine cross-bridge structure in Cs1A B. Secondary structure of Cs1A, by structural prediction results from AlphaFold. The cyestine residues are colored orange, displaying their side chains and the rest of the peptide in white</b></center>
+Paralysis and mortal effects of susceptible subjects are achieved via Cs1A inhibition on both high-voltage-activated (HVA) Cav channels and low-voltage-activated (LVA) Cav channels of susceptible targets by blocking the channels directly, resulting in impediment of fundamental nervous system responses in neuronal, muscular, and cardiac functions. (Specific site of inhibition depends on the concentration of neurotoxin).
+===Toxicity Verification===
+Cs1A is synthesized using the vector pET28a-G1M5-His-SUMO-Cs1A-GNA-His[Fig2B], of which is assembled using GoldenGate cloning and transformed into <i>E. coli</i> strain DH5ɑ. Colony PCR and sequencing is then carried out to verify the plasmid construct, of which is extracted and transformed into BL21(DE3) strain for expression. After IPTG induction and overnight incubation, the liquid culture is harvested and, after cell lysis, have an SDS-PAGE run. The results suggest that Cs1A had achieved soluble expression. After several unsuccessful purification attempts, the supernatant is treated directly by SUMO protease [Fig2C].
+<center><html><img src="https://static.igem.wiki/teams/5184/parts/cs1a-sumo.webp" width="600"/></html></center>
+<center><b>Fig2: (A) G1M5 tag allows secretion of the fusion protein into extracellular milieu (B) Plasmid construct pET28a-G1M5-His-SUMO-Cs1A-GNA-His (C) SDS-PAGE of supernatant and SUMO-treated supernatant, with supernatant of similarly treated supernatant of BL21(DE3) as control</b></center>
+The SUMO-digested supernatant's toxicity against ''T. urticae'' females is tested using a spraying method by Professor Huang from SCAU.
+Results from the toxicity assay suggests Cs1A to be highly toxic against ''T. urticae'', achieving an fatality of 92.73% within 72 hours.
+<center><html><img src="https://static.igem.wiki/teams/5184/parts/cs1a-lethality.webp" width="600"/></html></center>
+<center><b>Fig3: (A) ''T. urticae'' in their normal state, before being sprayed with treated supernatant (B) Dead ''T. urticae'' from spraying of treated supernatant (C) Survival plot of ''T. urticae'' being sprayed with supernatant containing Cs1A over 72 hours, CK is similarly processed supernatant of BL21(DE3), acting as a control (D) Lethality data of ''T. urticae'' being sprayed with supernatant over 24, 48, and 72 hours, CK is the similarly processed supernatant of BL21(DE3), acting as a control</b></center>
+==Part Collection==
+Our part collection provides a comprehensive list of venom peptides with a diverse range of molecular targets, and all displays satisfactory elimination efficacy during our testings [Fig7A&B].
+<center><html><img src="https://static.igem.wiki/teams/5184/parts/vp-lethality-v.webp" width="600"/></html></center>
+<center><b>Fig7: A. Survival plot of 6 venom peptides against female ''T. urticae'' using a spraying method, CK is induced liquid culture of BL21(DE3), of which acts as control D. Lethality data of 6 venom peptides over 24, 48, and 72 hours, CK is induced liquid culture of BL21(DE3), of which acts as control; data is the means of ± SD of three parallel replicate experiments</b></center>
+{|class="wikitable" style="margin:auto"
+|+ Our Part Collection
+|-
+!Current VP!!Venom Name!!Targeted Ion Channel!!New?!!Part Number!!Original Specie
+|-
+|||PpVP2S||Ca||New||BBa_K5184043||''Phytoseiulus persimilis''
+|-
+|||PpVP1S||Ca||New||BBa_K5184042||''Phytoseiulus persimilis''
+|-
+|||PpVP1F||Ca||New||BBa_K5184038||''Phytoseiulus persimilis''
+|-
+|||rCtx4||Na||||BBa_K5184021||''Phoneutria depilata''
+|-
+|✳️||Cs1A||Ca||||BBa_K5184032||''Calommata signata''
+|-
+|||HxTx-Hv1h||Ca, K||||BBa_K5184033||''Hadronyche versuta''
+|}