New pages

5 June 2025

• 12:4312:43, 5 June 2025 Immunoprecipitation (hist | edit) [2,125 bytes] ESO wikiadmin (talk | contribs) (Created page with "This is an original excerpt from MHE's digital labbook from 25 April 2025. {{Protokoll-Box}} = Immunoprecipitation = -       THP-1 Cells (WT, PPM1F KO (clone D7), PPM1F KO + PPM1F WT (clone C9), PPM1F KO+ PPM1F D360A (clone A5)) were count and 3x10⁶ cells were lysed using 1000 µl RIPA lysis buffer (10 µg/ml Aprotinin,10 µM Benzamidin, 5 µg/ml Leupepin, 1 µM PMSF, 10 nM pNPP, 2 µM cytochalasinD, cpd26, 1x Phosstop) -       Cells were vortexted, s...") Tag: Visual edit
• 12:2812:28, 5 June 2025 Bio-Rad GelDoc (hist | edit) [4,137 bytes] ESO wikiadmin (talk | contribs) (Created page with "= Bio-Rad GelDoc XR+ System - Overview = == What is the GelDoc XR+ System? == The GelDoc XR+ System from Bio-Rad is a reliable gel documentation system designed for high-quality imaging of nucleic acid and protein gels. This system combines proven CCD camera technology with versatile illumination options to provide consistent, publication-quality images for routine gel documentation needs. == Main Applications == === Nucleic Acid Gel Documentation === * '''Agarose ge...") Tag: Visual edit
• 12:2412:24, 5 June 2025 Bio-Rad ChemiDoc Touch (hist | edit) [2,807 bytes] ESO wikiadmin (talk | contribs) (Created page with "= Bio-Rad ChemiDoc Touch System - Overview = == What is the ChemiDoc Touch System? == The ChemiDoc Touch System from Bio-Rad is a versatile imaging system for documentation and analysis of gels and blots. It combines high-resolution CCD camera technology with intuitive touchscreen operation and enables capture of fluorescence, chemiluminescence, and visible light images. == Main Applications == === Gel Documentation === * '''Agarose gels:''' DNA/RNA electrophoresis w...") Tag: Visual edit
• 12:1712:17, 5 June 2025 Thermo Scientific Varioskan Flash eng (hist | edit) [4,117 bytes] ESO wikiadmin (talk | contribs) (Created page with "This page is also available in german 🇩🇪. = Varioskan Flash - Basic Operation Guide = == Overview == The Varioskan Flash is a multimode microplate reader for various detection methods (absorbance, fluorescence, luminescence, time-resolved fluorescence). This guide provides a basic overview - '''the manual remains essential for detailed protocols!''' == Preparation == === 1. Power on the instrument === * Activate main power...") Tag: Visual edit
• 12:1112:11, 5 June 2025 Thermo Scientific Varioskan Flash (hist | edit) [4,438 bytes] ESO wikiadmin (talk | contribs) (Created page with "Diese Seite ist auch auf Englisch 🇬🇧 verfügbar. = Varioskan Flash - Grundlegende Bedienung = == Überblick == Der Varioskan Flash ist ein Multimode-Mikroplatten-Reader für verschiedene Detektionsmethoden (Absorbanz, Fluoreszenz, Lumineszenz, Zeit-aufgelöste Fluoreszenz). Diese Anleitung bietet einen ersten Überblick - '''das Handbuch bleibt unverzichtbar für detaillierte Protokolle!''' == Vorbereitung == === 1. Ger...") Tag: Visual edit

3 June 2025

• 16:2216:22, 3 June 2025 S1 - Cell culture guidelines (hist | edit) [2,363 bytes] ESO wikiadmin (talk | contribs) (Created page with "'''Getting started:''' * Turn on hood, open bench  needs several minutes, wait for green light * Tie back hair, push back lose sleeves; disinfect hands & arms, put on gloves (can be reused) * Wipe down bench and window with 70% EtOH * Gather all material you need, spray with 70% EtOH and wipe down before placing under hood * Arrange items under hood towards the back of the bench ⇒Keep in mind that you should work a minimum of 15cm inward from the outside edge of th...") Tag: Visual edit
• 13:0313:03, 3 June 2025 Laborsicherheit (hist | edit) [6,165 bytes] ESO wikiadmin (talk | contribs) (Created page with "== '''Schutzkleidung''' == In den Laboren ist bei allen Arbeiten IMMER ein geschlossener Labormantel und eine Schutzbrille zu tragen. Besondere Vorsicht ist bei Arbeiten mit flüssigem Polyacrylamid (Gießen von SDS-PAGE-Gelen) und bei Arbeiten mit Säuren/Laugen walten zu lassen. Zusätzlich zu Labormantel und Schutzbrille sind hierbei Handschuhe zu tragen. == '''Gas''' == Laborgas ist zentral in Raum ML in einem Sicherheitsschrank untergebracht. Die Gasversorgung soll...") Tag: Visual edit

2 June 2025

• 09:2809:28, 2 June 2025 FBA-staining of bacteria (hist | edit) [1,326 bytes] ESO wikiadmin (talk | contribs) (Created page with "{{Protokoll-Mix|Inhalt=(5-(6)-carboxyfluorescein succinimidyl ester (CFSE, FAM SE, Fluorescein)<br>NHS-Biotin<br>PBS++ (PBS, 45 nM CaCl 2, 35 nM MgCl 2)<br>4% Paraformaldehyde (PFA)<br>Blocking solution (10% FCS in PBS ++)<br>PBS<br>Streptavidin-AlexaFluor647}} == Procedure == * Dilute 0.2 mg NHS-Biotin in 1 ml PBS (prewarm Biotin to RT before opening the tube) * Collect bacteria from plate in PBS, centrifuge for 4 min, 4000 rpm, and resuspend the pellet in 700 l PB...") Tag: Visual edit
• 09:0409:04, 2 June 2025 Gentamicin Protection Assay (hist | edit) [1,691 bytes] ESO wikiadmin (talk | contribs) (Created page with "== Procedure == * Aspirate cell culture medium with a pasteur pipette * Rince attaching cells carefully with cold PBS, aspirate PBS * Add 1.5 mL Trypsin/EDTA and study the detachment of the cells in the microscope * Inactivate Trypsin/EDTA with 3.5 mL medium, transfer the cell suspension into a 15 mL centrifuge tube * Pipette 20 mL of the cell suspension into a Neubauer counting chamber * Centrifuge the remaining cells at 600 rpm for 3 min * During centrifugation: Deter...") Tag: Visual edit
• 08:5308:53, 2 June 2025 Monitoring bacterial growth (hist | edit) [2,520 bytes] ESO wikiadmin (talk | contribs) (Created page with "{{Protokoll-Mix|Inhalt=Depending on the bacterium you want to analyse, you should determine beforehand: *Growth temperature *Shaking intensity *Generation time *Appropriate medium *Liquid or plate culture}} == Pre-culture == Streak out bacteria one to two days prior to the experiment: two days if you want to do a selection for single clones or if you have to incubate them on antibiotics. Addition of antibiotics usually hampers with the growth - for the determination o...") Tag: Visual edit
• 08:4908:49, 2 June 2025 Transformation of Neisseria gonorrhoeae (hist | edit) [1,000 bytes] ESO wikiadmin (talk | contribs) (Created page with "{{Protokoll-Mix|Inhalt=Gonococcal strain which is Opa-postive /Pili positive PPM medium (15g proteose pepton, 5g NaCl, 4g KH 2PO4 1g K2HPO4, 1g soluble starch, ad 1l H20 ph: 7.5) + vitamin mix cloned and sequenced analysed gonococcal DNA which contains the spectinomycin resistance cassette and the Neisserial DNA uptake sequence (DUS) (plasmid DNA}} == Procedure == * Ngo strain (O+/P+) were grown overnight (37°C) on GC agar plates in a humid atmosphere with 5% CO 2 * N...") Tag: Visual edit
• 08:3908:39, 2 June 2025 Transformation of plasmids in E. coli (hist | edit) [1,266 bytes] ESO wikiadmin (talk | contribs) (Created page with " == Procedure == * Before transformation, appropriate aliquots of competent bacteria should be thawn on ice. * Add the plasmid DNA to 100 μl competent E. coli in a snap-cap tube and mix well. * Incubate the samples 30 min on ice. * Transfer samples for 75 seconds to a 42°C water bath or heating block and quickly back on ice. * Add 1 ml LB-Medium and incubate the bacteria for 1h at 37°C (220 rpm). * Transfer the bacterial suspension from the snap-cap tube to Eppendorf...") Tag: Visual edit

30 May 2025

• 15:4615:46, 30 May 2025 InFusion-cloning (Fa. Clontech) (hist | edit) [711 bytes] ESO wikiadmin (talk | contribs) (Created page with "{{Protokoll-Mix|titel=Materials|Inhalt=InFusion Kit Becton-Dickinson<br>Aqua bidest<br>Linearised vector (pDNR-Dual), 100ng/1µl (~4900bp)<br>Fragment (10-50ng/µl)<br>-> Subsequent method: Transformation}} == Procedure == * fragment concentration (fragment : pDNR-Dual  2:1 ratio [fmol]) * solution of a dry-down reaction in 102 µl aqua bidest * add 14 µl 10x In-Fusion-buffer and 2 µl pDNR-Dual (200 ng) * disperse to 15 tubes (8 µl per tube) and add 0.5 -1 µl of...") Tag: Visual edit
• 15:4315:43, 30 May 2025 Cre-Lox recombination of plasmids (hist | edit) [1,238 bytes] ESO wikiadmin (talk | contribs) (Created page with "== Procedure == * Dilute Cre-recombinase [10 U/µl] with 1x Cre-recombinase-buffer 1:10 [1 U/µl] * Recombination reaction contains: ** 1 µl 10x Cre-recombination-buffer 6µl aqua bidest. ** 1 µl (100ng) donor vector (e.g. pDNR-dual gene X) ** 1 µl (200ng) acceptor vector (e.g. pLPS3’-EGFP) ** 2 µl Cre-recombinase * Incubation for 45 min at 37° C, meanwhile starting heating-unit * Heat inactivation for 10 min at 70° C and subsequent cooling to room temperature...") Tag: Visual edit
• 15:4015:40, 30 May 2025 Site directed mutagenesis (hist | edit) [1,879 bytes] ESO wikiadmin (talk | contribs) (Created page with "== Procedure == * Prepare the PCR reaction mix according to the hot start procedure. Include one negative control sample without Pfu polymerase (incubate sample at the lowest annealing temperature of your gradient) * Perform gradient PCR using the following thermal cycling conditions: {| class="wikitable" !Step !Temperature °C !Time !No. of cycles |- |Initial denauturation |94 |1-3 min |1 |- |Hot Start / add enzyme |94 |pause |1 |- |Denauturation |94 |20 sec | rowspan...") Tag: Visual edit
• 15:3315:33, 30 May 2025 Cloning of guideRNA-Oligo into pLentiCRISPRv2 (hist | edit) [2,019 bytes] ESO wikiadmin (talk | contribs) (Created page with "{{Protokoll-Mix|titel=Materials|Inhalt=gRNA Oligos (sense/antisense; designed using ChopChop)<br>Vector pBluescript_U6-MCS digested with BbsI (Plasmid #3468)<br>T4 DNA ligase; 10x Ligase buffer<br>E. coli NovaBlue}}")
• 15:3015:30, 30 May 2025 Cloning of guideRNA-Oligo into pBluescript U6-MCS (hist | edit) [2,000 bytes] ESO wikiadmin (talk | contribs) (Created page with "== Procedure == '''gRNA Oligo annealing''' * annealing reaction contains: 1 µl sense primer (stock solution 100 µM), 1 µl antisense primer (stock solution 100 µM), 5 µl NEB buffer 2 and 43 µl ddH₂O * Annealing reaction occurs in thermocycler with the corresponding program: {| class="wikitable" |95°C |4 minutes |- | colspan="2" |Start loop, 54x, 94°C, 1 min (-1°C/loop) |- |8°C |Store forever |} == Preparation of BbsI digested vector pBluescript_U6...") Tag: Visual edit
• 15:1815:18, 30 May 2025 Design of guideRNA-Oligos (gRNA) for CRISPR/Cas gen. editing (hist | edit) [1,268 bytes] ESO wikiadmin (talk | contribs) (Created page with "{{Protokoll-Mix|Inhalt= 20 mM dNTPs<br>10x Taq/Pfu buffer<br>2 Primers 10 μM<br> DNA template, 100 – 200 ng/μL<br>DNA polymerases (Pfu, Taq)}}") Tag: Visual edit: Switched
• 12:1312:13, 30 May 2025 Cloning of shRNA into lentiviral vector pLKO.1 (hist | edit) [2,225 bytes] ESO wikiadmin (talk | contribs) (Created page with "== Procedure == === Primer annealing === * annealing reaction contains: 1 µl sense primer (stock solution 100 µM), 1 µl antisense primer (stock solution 100 µM), 5 µl NEB buffer 2 and 43 µl ddH₂O * Annealing reaction occurs in thermocycler with the corresponding program:") Tag: Visual edit
• 12:0412:04, 30 May 2025 LIC Cloning (Ligation independent cloning) (hist | edit) [2,339 bytes] ESO wikiadmin (talk | contribs) (Created page with " == Procedure == Design primers compatible for cloning in vector containing the LIC sequence (e.g. pDNR Dual LIC) and perform PCR. Separate 4 µl of PCR reaction via agarose gel electrophoresis to check PCR product. Many unspecific bands besides the desired one require gel separation of the PCR sample and extraction of the desired band. If necessary, 2-3 PCR reactions can be pooled to gain more material. Add 10x NEB2 Buffer to the PCR sample to reach 1x end concentration...") Tag: Visual edit: Switched
• 11:2811:28, 30 May 2025 Designing PCR-Primers for LIC Cloning (Ligation independent cloning) (hist | edit) [2,695 bytes] ESO wikiadmin (talk | contribs) (Created page with " == Procedure == Delineate the coding sequence (full-length or partial sequence), which you want to amplify. Sense and antisense primers should have around 18 to 22 complementary bases, depending on the AT-content (there should be 9-10 Gs or Cs in the primer- cDNA complementary region). Both primers should ideally end with a 3’-GC clamp (two G or C bases). In the antisense primer, add a STOP codon, if you want to create a protein with an N- terminal tag; omit the STOP...") Tag: Visual edit
• 11:2311:23, 30 May 2025 Isolation of DNA from agarose gel (hist | edit) [1,295 bytes] ESO wikiadmin (talk | contribs) (Created page with "{{Protokoll-Mix|Inhalt= 20 mM dNTPs<br>10x Taq/Pfu buffer<br>2 Primers 10 μM<br> DNA template, 100 – 200 ng/μL<br>DNA polymerases (Pfu, Taq)}}") Tag: Visual edit: Switched
• 11:2111:21, 30 May 2025 PCR purification (hist | edit) [705 bytes] ESO wikiadmin (talk | contribs) (Created page with "{{Protokoll-Mix|Inhalt=TAE buffer (1x) 4.84 g Tris-Base, 1 mM EDTA, 1.14 mL acetic acid, fill 1 L with A.bidest. Agarose}}") Tag: Visual edit: Switched
• 10:0010:00, 30 May 2025 Setting up quantitative real-time PCR qRT-PCR (hist | edit) [1,115 bytes] ESO wikiadmin (talk | contribs) (Created page with "{{Pipetten-Checklist-8step}}") Tag: Visual edit
• 09:4109:41, 30 May 2025 PCR approach in 20 μL with hot-start (qualitative PCR) (hist | edit) [1,613 bytes] ESO wikiadmin (talk | contribs) (Created page with "{{Protokoll-Mix|Inhalt= The same as for PCR approach in 50 µL}}")

29 May 2025

• 18:1218:12, 29 May 2025 PCR approach in 50 μL with hot-start and/or touch-down (preparative PCR) (hist | edit) [1,801 bytes] ESO wikiadmin (talk | contribs) (Created page with "{{Protokoll-Mix|Inhalt=20 mM dNTPs 10x Taq/Pfu buffer 2 Primers, 10 μM DNA template, 100 – 200 ng/μL DNA polymerases (Pfu, Taq)}} == Procedure == As usually more than one PCR sample is run simultaneously, reaction and enzyme mix are prepared separately. The enzyme mix is added to the reaction mix after starting the PCR and after pre-heating the reaction mix to 94 ºC (hot start). A typical 50 μL approach that yields enough material for later cloning procedures...") Tag: Visual edit
• 18:0418:04, 29 May 2025 Design principles for PCR primers used for amplification and cloning of cDNA (hist | edit) [2,490 bytes] ESO wikiadmin (talk | contribs) (Created page with "'''Restriction Enzyme Sites:''' For conventional cloning with restriction enzymes, the recognition sites are added to the 5’ end of the primer. Check that the involved '''restriction enzymes do NOT cut within the cloned cDNA''' and that they do '''NOT cut the vector outside the intended position'''. Make sure to preserve the reading frame, if the DNA is cloned 3’ or 5’ of existing ORFs (e.g. GFP) in the vector. Add 3 to 4 meaningless nucleotides (e.g. ATAA-) at the...") Tag: Visual edit
• 17:5617:56, 29 May 2025 Agarose gel electrophoresis (hist | edit) [1,341 bytes] ESO wikiadmin (talk | contribs) (Created page with "{{Protokoll-Mix |titel=PCR Reaction mix (Pipett scheme) |TAE buffer (1x) 4.84 g Tris-Base, 1 mM EDTA, 1.14 mL acetic acid, fill 1 L with A.bidest. Agarose }}")
• 16:1816:18, 29 May 2025 Vorlage:Homepage-Grid (hist | edit) [1,174 bytes] ESO wikiadmin (talk | contribs) (Created page with "<div style="display: grid; grid-template-columns: 1fr 1fr; gap: 20px; margin: 20px 0;"> <div style="grid-column: 1;"> {{Colored-Box |title={{{title1|Titel 1}}} |content={{{content1|Inhalt Box 1}}} |background={{{bg1|#e8f4fd}}} |border={{{border1|#3366cc}}} |link={{{link1|}}} |link-text={{{linktext1|Mehr →}}} }} </div> <div style="grid-column: 2;"> {{Colored-Box |title={{{title2|Titel 2}}} |content={{{content2|Inhalt Box...")
• 16:1816:18, 29 May 2025 Vorlage:Colored-Box (hist | edit) [707 bytes] ESO wikiadmin (talk | contribs) (Created page with "<div class="colored-box" style="background: {{{background|#f8f9fa}}}; border: 1px solid {{{border|#a2a9b1}}}; border-radius: 4px; padding: 16px; margin: 10px 0; box-shadow: 0 1px 3px rgba(0,0,0,0.1);"> {{#if:{{{title|}}}|<h3 style="margin-top: 0; color: {{{title-color|#0645ad}}}; border-bottom: 1px solid {{{border|#a2a9b1}}}; padding-bottom: 8px; margin-bottom: 12px;">{{{title}}}</h3>}} <div style="color: {{{text-color|#333}}};"> {{{content|Box-Inhalt hier}}} <...")
• 16:1516:15, 29 May 2025 Vorlage:Tip (hist | edit) [170 bytes] ESO wikiadmin (talk | contribs) (Created page with "<div style="border-left: 4px solid #8b5cf6; background: #f5f3ff; padding: 12px; margin: 16px 0; border-radius: 2px;"> <strong>💡 Tipp:</strong> {{{1|Tipp-Text}}} </div>")
• 16:1416:14, 29 May 2025 Vorlage:Info (hist | edit) [179 bytes] ESO wikiadmin (talk | contribs) (Created page with "<div style="border-left: 4px solid #00af89; background: #f0fdf4; padding: 12px; margin: 16px 0; border-radius: 2px;"> <strong>ℹ️ Info:</strong> {{{1|Informationstext}}} </div>")
• 16:1416:14, 29 May 2025 Vorlage:Warning (hist | edit) [174 bytes] ESO wikiadmin (talk | contribs) (Created page with "<div style="border-left: 4px solid #d73027; background: #fdf2f2; padding: 12px; margin: 16px 0; border-radius: 2px;"> <strong>⚠️ Warning:</strong> {{{1|Warntext}}} </div>")
• 16:0916:09, 29 May 2025 Vorlage:Note (hist | edit) [174 bytes] ESO wikiadmin (talk | contribs) (Hinweisbox)
• 15:4415:44, 29 May 2025 Vorlage:Print-Button (hist | edit) [1,004 bytes] ESO wikiadmin (talk | contribs) (Print/Export-Button-Vorlage erstellt)
• 15:1015:10, 29 May 2025 Colony PCR (hist | edit) [1,640 bytes] ESO wikiadmin (talk | contribs) (Created page with "Reaction mix: H₂O                                         16.5 μL 10x Taq/Pfu buffer                       2 μL Primer 1                                    0.4 μL (10 pmol) Primer 2                                    0.4 μL (10 pmol) dNTP-Mix                                  0.2 μL Taq polymerase                        0.5 μL total              ...") Tag: Visual edit

21 May 2025

• 14:1414:14, 21 May 2025 Restriction digest of plasmid DNA (hist | edit) [1,054 bytes] ESO wikiadmin (talk | contribs) (Created page with "{| class="wikitable" |+ !Materials |- |Restriction enzyme stock (–20°C) |- |Appropriate 10x enzyme buffer (–20°C) |- |Sterile dd H₂O |- |Depending on the digestion '''(optional)''': '''''BSA (bovine serum albumin)''''': To ensure 100% activity of the enzymes, 100 µg/ml BSA should be added (stored at –20°C) |} == Procedure for analysis purposes == * 300 ng of DNA samples (e.g. control digest of plasmid minipreps) * 1 µl appropriate enzyme buffer (1...") Tag: Visual edit
• 14:1114:11, 21 May 2025 Plasmid-Miniprep (Birnboim – Dooley protocol) (hist | edit) [1,327 bytes] ESO wikiadmin (talk | contribs) (Created page with "{| class="wikitable" |+ !Materials |- |Buffer P1: Solve 6.055 g Tris Base and 3.722g EDTA x 2H₂O in 800 ml H₂0. Adjust pH to 8.0 with 1M HCl, fill up to 1L. Per 1 ml buffer P1, add 100 µg RNase A. Store at 4°C. |- |Buffer P2: Solve 8.0 g NaOH in 950 ml H₂0. Add 50 ml 20% SDS. Store at RT. |- |Puffer P3: 294.45g KAc in 500 ml H₂O. Adjust pH to 5.5 with glacial acetic acid (about 110 ml acid needed), fill up to 1L with H<sub>...") Tag: Visual edit

20 May 2025

• 15:2715:27, 20 May 2025 Vorlage Klonierungsprojekt (hist | edit) [2,298 bytes] ESO wikiadmin (talk | contribs) (Created page with "<noinclude> == Vorlage für Klonierungsprojekte == Diese Seite dient als Vorlage für neue gentechnische Arbeiten im Labor (z. B. PCR-Klonierungen). Kopiere den folgenden Inhalt in eine neue Wiki-Seite und passe ihn projektbezogen an. '''Hinweis:''' Alle Datumsangaben, Enzyme, Vektoren etc. bitte entsprechend aktualisieren.</noinclude> == Projekttitel == ''(z. B. Klonierung von GFP-tagged PAK1 in pcDNA3.1)'' * Startdatum: __.__.20__ * Bearbeiter: Benutzer:DeinN...") Tag: Visual edit
• 15:1615:16, 20 May 2025 Flow chart of a PCR-based cloning project (hist | edit) [3,199 bytes] ESO wikiadmin (talk | contribs) (Created page with "== Experimenteller Ablaufplan eines klassischen PCR-basierten Klonierungsprojekts == ''(LIC-basiertes Klonieren kann in vergleichbarer Zeit mit ähnlichen Schritten durchgeführt werden)'' === Montag === * PCR (5 × 50 µl Reaktionen im Temperaturgradienten) * 5 µl jeder PCR-Reaktion auf Agarosegel laden, Produktgröße & Qualität kontrollieren * 2–3 Proben kombinieren (3 × 45 µl), 5 µl DpnI hinzufügen, 1 h bei 37 °C inkubieren * 5-faches Volumen Puffer PB (...") Tag: Visual edit: Switched
• 15:0915:09, 20 May 2025 Fluorescent Staining of Cryosections (hist | edit) [881 bytes] ESO wikiadmin (talk | contribs) (Created page with "{| class="wikitable" |+ !Materials |- |PBS pH 7.4 |- |Blocking buffer (1% BSA, 1% serum and 0.1% Triton X-100 in PBS) |- |Corresponding 1st and 2nd antibodies |- |Barrier pen |- |Mounting medium |} === Procedure: === * Thaw the slides at room temperature for 10-20 min * The slides are washed for 10 min in PBS * Block non-specific staining by incubating samples in blocking buffer for 30 minutes at RT * Surround the tissue with a hydrophobic barrier using a barrier pen...") Tag: Visual edit
• 15:0615:06, 20 May 2025 Tissue/embryo preparation fo cryosectioning (hist | edit) [1,081 bytes] ESO wikiadmin (talk | contribs) (Created page with "{| class="wikitable" |+ !Materials |- |PBS pH 7.4 |- |4% PFA in PBS |- |10%, 20% and 30% sucrose solution in PBS |- |OCT Tissue-Tek |- |Histology moulds |- |Pre-coated glass slides |- |Dry ice |} === Procedure: === * Tissues/ anesthetized embryos are dissected and placed into 4% PFA solution overnight at 4° C * The next day the specimen is washed with PBS and transferred to a 10% sucrose solution for 3 h at 4° C (keep at 4°C until specimen sinks) * The sample is tra...") Tag: Visual edit
• 15:0315:03, 20 May 2025 Bacterial invasion assay by flow cytometry (hist | edit) [1,704 bytes] ESO wikiadmin (talk | contribs) (Created page with "{| class="wikitable" |+ !Materials (for 6 cm dishes) |- |CFSE |- |FACS buffer (1% (F)CS in PBS, 50-100 mL (ice-cold) |- |Trypsin/EDTA (1mL/dish) |- |Medium with serum according to cell type (3mL/dish) |- |15 mL PP falcon tubes |- |Trypan blue solution, 0.4 mg/mL |- |Eppendorf tubes 1.5mL (1 per dish) |} === Procedure === Bacteria: * 2 days before the experiment, streak bacteria from glycerol stock on selective GC or TSB agar plates (with antibiotics when needed) and in...") Tag: Visual edit
• 09:5709:57, 20 May 2025 Staining of cells for flow cytometry (hist | edit) [1,663 bytes] ESO wikiadmin (talk | contribs) (Created page with "{| class="wikitable" |+ ! ! ! ! |- |FACS buffer: |1xPBS FCS (heat-inactivated, final concentration: 5%) 5% Natriumazid (final concentration: 0.1%) | | |- |1st antibody: |primary antibody (approx. dilution 1:200) | | |- |2nd antibody: |secondary antibody (approx. dilution 1:500) fluorescence- labelled | | |- |controls: |sample with irrelevant primary antibody and secondary antibody sample with secondary antibody only if possible untransfected cells stained with both antib...") Tag: Visual edit
• 09:5409:54, 20 May 2025 Scanning electron microscopy (SEM) (hist | edit) [2,243 bytes] ESO wikiadmin (talk | contribs) (Created page with "{| class="wikitable" |+ !Materials |- |'''Fixation buffer''': 3% Formaldehyde, 2% Glutardialdehyde, 10 mM CaCl₂, 10 mM MgCl₂, 90 mM Sucrose in 100 mM HEPES, pH 7.2 |- |'''Washing Buffer''': 10 mM CaCl₂, 10 mM MgCl₂, 90 mM Sucrose in 100 mM HEPES, pH 7.2 |- |'''HEPES buffer:''' 100 mM, pH 7.2 |- |'''Graded ethanol series:''' 30%, 50%, 70%, 90%, 100% ethanol p.a. |} === Procedure: === '''1A. ''Organs''''' of infected animals are...") Tag: Visual edit
• 09:4309:43, 20 May 2025 OPTIC (Opa protein triggered integrin clustering) (hist | edit) [2,588 bytes] ESO wikiadmin (talk | contribs) (Created page with "{| class="wikitable" |+ !Materials |- |1x PBS |- |Trypsin/EDTA |- |GC-Agar plates with CAM/ERM and without antibiotics Coverslips (round, 12 mm) |- |24 well plate |- |HEK culture medium (DMEM + 10% CS) Suspension medium (DMEM + 0.25% BSA) 4% paraformaldehyde (PFA) in PBS |- |Permeabilization solution (0.4% Triton-X-100 in PBS) Blocking solution (10% heat inactivated CS in PBS) Mounting medium |} === Procedure === ==== '''Day1:''' ==== ==== Seed HEK293T cells 1:40 in 6...") Tag: Visual edit
• 09:3909:39, 20 May 2025 Live cell microscopy (hist | edit) [1,282 bytes] ESO wikiadmin (talk | contribs) (Created page with "=== Preparation of culture dishes === * In 3.5 cm culture dishes (Sarstedt 83.1800 35x10 mm) a hole is drilled with 14 mm in diameter (will be done by the uni garage) * Before sticking the coverslips (Menzel 24 mm, Stärke 1,5; CB00240RAC20MNZ#0) to the dishes spray them with 70% ethanol and wipe with a KimWipe tissue * The coverslips are pretreated as following: ** Wash with a mixture of 50% v/v Aceton and 50% v/v EtOH ** Wash with 1xPBS ** Wash with MilliQ water ** Dr...") Tag: Visual edit

7 May 2025

• 15:4515:45, 7 May 2025 Lab Etiquette (ENG) (hist | edit) [19,216 bytes] ESO wikiadmin (talk | contribs) (Created page with "'''<div style="border: 1px solid #ccc; background: #f9f9f9; padding: 1em; margin-bottom: 1em;"> '''<span style="font-size:120%; font-weight:bold;">Welcome to the lab – think together, act together!</span>''' A well-functioning lab doesn’t rely solely on rules but on mutual awareness and shared responsibility. Especially for newcomers, it’s better to ask one question too many than to do the wrong thing silently. If you notice that something is running out – let p...")
• 15:2815:28, 7 May 2025 Laborbuchführung (hist | edit) [3,248 bytes] ESO wikiadmin (talk | contribs) (Created page with "'''Diese Seite ist auch auf Englisch verfügbar.''' = Laboratory Bookkeeping Guide = == Ein praxisorientierter Leitfaden für sauberes und effizientes Arbeiten im Forschungslabor == === Warum Laborbuchführung wichtig ist === Saubere Buchführung im Labor ist kein lästiger Formalismus – sie ist ein Grundpfeiler wissenschaftlicher Integrität. [...] === Grundprinzipien === # '''Nachvollziehbarkeit''' # '''Unveränderbarkeit''' # '''Z...")
• 15:2715:27, 7 May 2025 Laboratory Bookkeeping Guide (hist | edit) [2,796 bytes] ESO wikiadmin (talk | contribs) (Created page with "'''This page is also available in German.''' = Laboratory Bookkeeping Guide = == A practical guide to structured and efficient lab documentation == === Why lab bookkeeping matters === Clean lab documentation isn’t just bureaucracy – it’s a cornerstone of scientific integrity. [...] === Core principles === # '''Traceability''' # '''Immutability''' # '''Timeliness''' # '''Structure''' === Analog or digital? === [...] === What to include =...") Tag: Visual edit