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當(dāng)前位置 > 產(chǎn)品目錄 > 試劑 > 植物試劑 > FtsH3 + FtsH10 | plant fts metallo-protease H3 + H10
FtsH3 + FtsH10 | plant fts metallo-protease H3 + H10
英文名稱(chēng):FtsH3 + FtsH10 | plant fts metallo-protease H3 + H10總訪問(wèn):303
國(guó)產(chǎn)/進(jìn)口:進(jìn)口半年訪問(wèn):2
產(chǎn)地/品牌:agrisera產(chǎn)品類(lèi)別:植物試劑
規(guī)       格:AS07204 最后更新:2024-12-5
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product information
background

One of the several classes of mitochondrial proteases is membrane bound, ATPdependent FtsH protease. Their function is very important for the control of protein quality and quantity by degradation of unassembled subunits. Other names: AtFtsH3, cell division protease ftsH homolog 3, mitochondrial, AtFtsH10, cell division protease ftsH homolog 10, mitochondrial

immunogen

KLH-conjugated peptide dereived from sequences of Arabidopsis thaliana FtsH3 and FtsH10 with localization to mitochondria Q84WU8, At2g29080 and Q8VZI8, At1g07510

antibody format

rabbit

polyclonal

affinity purified serum, in PBS pH 7.4

lyophilized

quantity

200 µg

for reconstitution add 100 µl of sterile water.

storage

store lyophilized/reconstituted at -20°C; once reconstituted make aliquots to avoid repeated freeze-thaw cycles. Please, remember to spin tubes briefly prior to opening them to avoid any losses that might occur from lyophilized material adhering to the cap or sides of the tubes.

tested applications

western blot (WB), Blue-native (2D BN/SDS-PAGE)

related products

AS07 205 | anti-FtsH4 | plant fts metallo-protease H4

AS07 251 | anti-FtsH10 | plant fts metallo-protease H10

additional information

Blue-native (2D BN/SDS-PAGE) methodology is described in Piechota et al. 2010

application information
recommended dilution

1 : 500- 1: 1000 with standard ECL (WB)

expected | apparent MW

80 kDa

confirmed reactivity

Arabidopsis thaliana

predicted reactivity

Arabidopsis thaliana

not reactive in

no confirmed exceptions from predicted reactivity known in the moment

additional information

to be added when available

selected references

Piechota et al. (2010). Identification and characetization of high-molecular-weight complexes fromed by m-AAA proteases and prohibitins in mitochondria of Arabidopsis thaliana. In press.


application example

total protein from Arabidopsis thaliana mitochondria (20 µg) were separated on 10% acrilamide gel and electrophoresis prepared according to Schägger and von Jagov (Anl. Biochem., 1987, 166:368-379). After running the gel, proteins were transferred to nitrocellulose membrane using wet transfer (0.22% CAPS, pH 11). Transfer was checked by Ponceau S staining. Blot was destained by several quick washings in distilled water and 1 washing in 1X TBS (10 mM T pH 7.5, 150 mM NaCl) (10-15 min.).Blot was blocked by 1.5 hour in 5% milk in TBST (1X TBS, 0,1 20) After blocking blot was washed quickly twice in TBST and incubated 2 hours with primary antibody (dilution 1: 1000 TBST (dilution 1:1000). Washing: two quick washings in TBST and 3 x 10 min. washings in TBST. Then blot was incubated 45-60 min. with a secondary anti-rabbit antibodies conjugated to peroxidase (Sigma, dilution 1:10000) in TBST. Washing: as above. After washing blot was incubated 1-2 min. in ECL solution and exposed to Kodakautoradiography film. Exposure time was 15-60 seconds.

Mitochondria were isolated as described by Urantowka et al. (Plant Mol Biol, 2005, 59:239-52). Mitochondrial pellets were suspended in 1X Laemmli buffer (5% beta-mercaptoetanol, 3.7% glycerol, 1.1% SDS, 23 mM Tris-HCl pH 6.8, 0.01% bromophenol blue), heated (95 ºC, 5 min.) and centrifuged (13000rpm, 1 min.).

Courtesy Dr. J. Piechota



western blot detection using anti-FtsH3/10 antibodiesbio-equip.com
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