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F-actinF-actin
β-actinβ-actin
actin基因actin gene
α-SM-actinα - smooth muscle - actin
actin結合活性actin binding activity
β-actin基因β-actin gene
-βactin啟動(dòng)子β-actin promoter
雞β-actin啟動(dòng)子Chicken β -actin promoter
EMA、Actin、S-100、ER陰性;Negatived for EMA,Actin,S-100,ER;
標記F-actin,熒光顯微鏡下觀(guān)察。F-actin was labled and examined using fluorescence microscope.
高糖組F-actin熒光強度為對照組的44.5%；High glucose can decrease the fluorescent intensity of F-actm to 44.5%25 (p<0.01);
MOMA-2表達增加,SM-actin表達降低(P<0.05)。Even,upregulation of MOMA-2 and downregulation of SM-actin were also detected in latter(P<0.05).
電離輻射對血管內皮細胞骨架蛋白F-actin影響的激光共聚焦顯微鏡觀(guān)察The Observation of the Influence of Ionizing Radiation on the Image of F-actin in Vascular Endothelial Cells with Confocal Laser Scanning Microscope
結果表明,LIM結構域2在hhLIM與actin相互作用及調節actin細胞骨架組構中起決定性作用.In conclusion, LIM domain 2 at the C-terminus of hhLIM plays a central role in F-actin polymerization and cytoskeleton stabilization, whereas the first LIM domain is essential for the nuclear localization of hhLIM.
其ANA以核膜型為主 (7 14 ) ; AIH患者ANA抗體未見(jiàn)特定的熒光類(lèi)型 ,而抗 Actin僅見(jiàn)于A(yíng)IH者。No specific ANA pattern were seen in AIH by IIF, and anti Actin was present only in patients with AIH.
4Hz、12Hz和20Hz的100dB的次聲作用30min/d后,可誘導F-actin表達的增強,這種改變在8h后仍未見(jiàn)減弱。F-actin expression can be increased in osteoblast MC3T3 exposed 30min/d by low intensity infrasound with output intensity of 100dB and frequency of 4Hz,12Hz,20Hz. The expression increasing of F-actin still can be founded at the 8th hour after exposed under the low intensity infrasound.
通過(guò)PCR技術(shù) ,我們從文庫中釣取到EGP、2 3kD膜蛋白、Actin和GCP的cDNA ,其中GCP基因為低豐度表達基因。By using PCR we obtained the cDNAs of EGP,23KD membrane protein,Actin and GCP from our cDNA libraries,GCP is a low|abundant expressed gene.
和a一SMA(a一smooth musele actin)的表達。 5反轉錄聚合酶鏈反應(reverse transcription一polymerase ehain reaction，mRNA expressions of TGF-B1 and PPAR r were detected by Reverse transcription-polymerase chain reaction (RT-RCR).
免疫組織化學(xué)染色結果顯示：Vimentin、Actin標記細胞呈陽(yáng)性反應。 Desmin、AACT、EMA、Cytokeratin和S－100標記為陰性。The results revealed that the cells were positive for vimentin, actin and negative for desmin, AACT, EMA, cytokeratin and S-100protein.
免疫組化結果:瘤細胞desmin及vimentin呈彌漫強陽(yáng)性表達,actin、CD34、ER和PR染色稍弱、呈灶狀分布,而S-100蛋白、NF和CK均陰性。Immunohistochemically, the tumor cells were strong positive for vimentin and desmin, only local positive for CD34, ER and PR, but all tumor cells were negative for S-100 protein, NF and CK.

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