XIE/2:2026/Jan: Difference between revisions

Latest revision as of 12:55, 28 January 2026

1.13[edit]

Synthesis of Anti-Oligo

抗体还原[edit]

取2 ul(1mM) TCEP,用 PBS(7.4) 稀释至 20 ul(100uM),取 5 ul稀释后的 TCEP ，加入 85 ul PBS(7.40)，涡旋混匀---TCEP溶液pH过低提前中和
取2 ul(50uM)抗体，用 PBS（pH 7.4）稀释至 10 ul（10uM），将 TECP 的 PBS 缓冲液加入其中，37℃ 孵育 2 h.
取1 ul(50uM)抗体，用 PBS（pH7.4）稀释至 8 ul，作为 C 组

偶联[edit]

将孵育好的溶液用 PBS(6.5) 洗涤4次（10000g 3.5min），均分样品（A.B）----buffer pH 6.5避免后续加入的Mal被水解（碱性易水解）
A（共混组）：向 A 中加入 5 ul(100uM) 的 Mal-PEg-DBCO 和 1 ul(1mM) Azide-ssDNA，室温避光孵育 4 h.
B（依次组）：1）向 B 中加入 5 ul(100uM) 的 Mal-PEg-DBCO，室温避光孵育 2 h. 2)孵育结束后，向其加入1 ul(1mM) Azide-ssDNA，室温避光孵育 2 h.

验证[edit]

强还原断开轻重链：向A、B、C中加入对应量的蛋白 loudingbuffer ，再各加入1 ulβ-巯基乙醇，100℃煮 10m in
10% SDS-Page.

1.19[edit]

incubation[edit]

DNA samples were stratified by thiolation status into two primary groups: thiolated DNA (bearing a thiol modification) and non-thiolated DNA (without thiol modification). Within each primary group, samples were further subdivided by phosphate-buffered saline (PBS) pH, yielding subgroups at pH 5.5, 6.5, 6.7, 6.8, 7.0, 7.5, and 8.5. PBS solutions were prepared and adjusted to the target pH and verified with a calibrated pH meter at room temperature.

S1 (100 μM)	S2 (100 μM)	TFO (100 μM)	Buffer
2 μl	2 μl	2 μl	194 μl

FRET[edit]

Method：Samples were measured in Cy3 and Cy5 channels using appropriate excitation/emission filters under constant instrument settings.

1.20[edit]

Antibody reduction[edit]

Dilute 2 µL of antibody stock with 1× PBS to 10 µL (10 µM).
Prepare a TCEP working solution by diluting 1.5 µL of 100 µM TCEP with 1× PBS to 90 µL.
Mix the 10 µL antibody with 90 µL TCEP working solution and incubate at 37°C for 2.5 h (final antibody ≈1 µM; TCEP ≈1.5 molar equivalents).
Purify the reduced antibody by three rounds of buffer exchange into 1× PBS.

Antibody functionalization with DBCO[edit]

Add 5 µL of Mal‑PEG4‑DBCO (100 µM) to the purified, reduced antibody and incubate at 37°C for 2 h (5 eq).

Antibody conjugation to oligo[edit]

Add 5 µL of Azide‑Oligo (100 µM) to the DBCO‑modified antibody and incubate at 37°C for 2 h to complete the strain‑promoted azide‑alkyne cycloaddition (SPAAC) coupling (5 eq).

Native-page[edit]

Analyze reaction products by non‑denaturing electrophoresis using 7.5% native PAGE.
Marker、Control（antibody）、Antibody-Oligo、Antibody-DNA、Marker

Conclusion :Nativepage is not a good chose antibody conjugation

1.21[edit]

Native-page[edit]

Samples(1.20 antibody with oligo) and controls were analyzed by native polyacrylamide gel electrophoresis (PAGE) using a 3–5% stacking gel and a 12.5% resolving gel.
Marker、Control（antibody）、Antibody-Oligo、Antibody-DNA、Marker

1.22[edit]

1.28[edit]

抗体偶联[edit]

平均偶联数量测量[edit]

双波长法计算标记度（Degree of Labeling, DoL）

以下公式采用 A280 和 A260 的吸光度值，通过校正 DNA 在 280 nm 处的贡献来计算抗体浓度、核酸浓度及最终的平均偶联数（DoL）。

CAb = [A280 − CF_DNA,280·A260] / εAb,280·L
CDNA = A260 / εDNA,260·L
DoL = CDNA / CAb、

L 光程这里为 1；A280，A260 样品吸光度；
CF_DNA,280·A260 “纯DNA”在同缓冲下测得的比值 A280/A260，用来估算DNA在280的交叉吸收；
εAb,280 抗体消光系数，本抗体为2.3865×10^5 M⁻¹·cm⁻¹；
εDNA,260 Oligo消光系数，该Oligo(TTTTCTCCTCTCTCCTCCTCTT，5'Azide)为 1.698×10^5 M⁻¹·cm⁻¹；

@@ Line 1: / Line 1: @@
 <div style="color: black !important; font-family: 'Times New Roman', SimSun, serif !important, line-height:1.5;">
 ==1.13==
+<big><span>Synthesis of Anti-Oligo
 ===抗体还原===
 *取2 ul(1mM) TCEP,用 PBS(7.4) 稀释至 20 ul(100uM),取 5 ul稀释后的 TCEP ，加入 85 ul PBS(7.40)，涡旋混匀---TCEP溶液pH过低提前中和
@@ Line 13: / Line 14: @@
 *10% SDS-Page.
 [[File:AOC_1.13.png|thumb|center|600px]]
 ==1.19==
 ===incubation===
@@ Line 21: / Line 23: @@
 | 2 μl || 2 μl || 2 μl || 194 μl
 |}
+===FRET===
+*Method：Samples were measured in Cy3 and Cy5 channels using appropriate excitation/emission filters under constant instrument settings.
+[[File:FRET-pH-260119.png|thumb|center|400px]]
+==1.20==
+===Antibody reduction===
+#Dilute 2 µL of antibody stock with 1× PBS to 10 µL (10 µM).
+#Prepare a TCEP working solution by diluting 1.5 µL of 100 µM TCEP with 1× PBS to 90 µL.
+#Mix the 10 µL antibody with 90 µL TCEP working solution and incubate at 37°C for 2.5 h (final antibody ≈1 µM; TCEP ≈1.5 molar equivalents).
+#Purify the reduced antibody by three rounds of buffer exchange into 1× PBS.
+===Antibody functionalization with DBCO===
+*Add 5 µL of Mal‑PEG4‑DBCO (100 µM) to the purified, reduced antibody and incubate at 37°C for 2 h (5 eq).
+===Antibody conjugation to oligo===
+*Add 5 µL of Azide‑Oligo (100 µM) to the DBCO‑modified antibody and incubate at 37°C for 2 h to complete the strain‑promoted azide‑alkyne cycloaddition (SPAAC) coupling (5 eq).
+===Native-page===
+*Analyze reaction products by non‑denaturing electrophoresis using 7.5% native PAGE.
+*Marker、Control（antibody）、Antibody-Oligo、Antibody-DNA、Marker
+[[File:Ab-Oligo Native 7.5 2026-01-23.jpg|thumb|center|400px]]
+Conclusion :Nativepage is not a good chose antibody conjugation
+==1.21==
+===Native-page===
+*Samples(1.20 antibody with oligo) and controls were analyzed by native polyacrylamide gel electrophoresis (PAGE) using a 3–5% stacking gel and a 12.5% resolving gel.
+*Marker、Control（antibody）、Antibody-Oligo、Antibody-DNA、Marker
+[[File:Ab-Oligo_Native4-12.5_2026-01-23.jpg|thumb|center|400px]]
+==1.22==
+==1.28==
+===抗体偶联===
+===平均偶联数量测量===
+*双波长法计算标记度（Degree of Labeling, DoL）
+以下公式采用 A280 和 A260 的吸光度值，通过校正 DNA 在 280 nm 处的贡献来计算抗体浓度、核酸浓度及最终的平均偶联数（DoL）。
+#CAb = [A280 − CF_DNA,280·A260] / εAb,280·L
+#CDNA = A260 / εDNA,260·L
+#DoL = CDNA / CAb、
+*L 光程 这里为 1；A280，A260 样品吸光度；
+*CF_DNA,280·A260 “纯DNA”在同缓冲下测得的比值 A280/A260，用来估算DNA在280的交叉吸收；
+*εAb,280 抗体消光系数，本抗体为2.3865×10^5 M⁻¹·cm⁻¹；
+*εDNA,260 Oligo消光系数，该Oligo(TTTTCTCCTCTCTCCTCCTCTT，5'Azide)为 1.698×10^5 M⁻¹·cm⁻¹；
+===SDS-page验证偶联结果===

Latest revision as of 12:55, 28 January 2026

1.13[edit]

抗体还原[edit]

偶联[edit]

验证[edit]

1.19[edit]

incubation[edit]

FRET[edit]

1.20[edit]

Antibody reduction[edit]

Antibody functionalization with DBCO[edit]

Antibody conjugation to oligo[edit]

Native-page[edit]

1.21[edit]

Native-page[edit]

1.22[edit]

1.28[edit]

抗体偶联[edit]

平均偶联数量测量[edit]

SDS-page验证偶联结果[edit]