Protocols

Media preparation protocol

Consistent media is the foundation of reproducible tissue culture. This protocol walks through weighing, dissolving, pH adjustment, dispensing, and autoclaving — with a sample Murashige and Skoog (MS) formulation and notes on recording each batch as an xPlant media recipe.

These are reference steps only — not a substitute for validated lab-specific procedures. Verify formulations against authoritative sources and your own experimental data before use.

Reference: MS basal medium (1 L)

Murashige and Skoog (1962) is the most widely used basal medium in tissue culture. The following table is a quick reference — use your lab's validated recipe or a quality premix where available.

Component	Amount	Note
Macro salts (MS premix)	4.4 g	Or weigh individual salts
Sucrose	30 g	Standard; reduce for some species
Myo-inositol	100 mg	Often included in premix
Thiamine HCl	0.1–1 mg	Often included in premix
Agar	7–8 g	Omit for liquid culture
Distilled water	To 1 L
pH	5.7–5.8	Adjust before autoclaving

Preparation steps

1
Gather materials
Analytical balance, distilled or deionised water, volumetric flask (1 L), magnetic stirrer + hotplate, pH meter, KOH or HCl for pH adjustment, agar (if solidifying), media salts and PGRs.
2
Dissolve salts
Add ~800 mL of distilled water to the flask. Weigh each macro- and micronutrient salt and dissolve in order of concentration (macros first). Stir gently; some salts may need gentle heat to dissolve fully.
3
Add sugar and vitamins
Add sucrose (typically 30 g/L for MS). Add vitamins (thiamine, glycine, myoinositol) if not included in a premix. Stir to dissolve.
4
Add plant growth regulators
Add PGRs (auxins, cytokinins) last before pH adjustment. Many PGRs are prepared as stock solutions (1000× or 10 000×) dissolved in KOH or ethanol — add the calculated volume from stock.
5
Adjust pH
Calibrate your pH meter. Adjust to pH 5.7–5.8 (or protocol-specific target) using 1 M KOH to raise or 1 M HCl to lower. pH will shift slightly on autoclaving — stop at 5.8 if autoclaving a solidified medium.
6
Add agar (solid media)
Bring volume to 1 L. Add agar (typically 7–8 g/L for standard solid media). Stir on hotplate until agar is fully suspended — it will not dissolve until autoclaved.
7
Dispense into vessels
Pour ~20–25 mL per culture tube or jar before autoclaving. Leave caps loose or use autoclave-safe vented caps. Do not overfill — agar expands slightly and needs headspace.
8
Autoclave
121 °C, 15 psi, 20 minutes (liquid cycle). Allow to cool to ~50–55 °C before pouring plates or adding heat-sensitive additives. Solidified media in vessels can cool in a rack.
9
Cool and store
Allow to solidify at room temperature. Inspect vessels for unusual colour, particulates, or contamination before use. Store at 4 °C for up to 4 weeks or at room temperature for up to 2 weeks (sealed, dark).

Logging batches in xPlant

xPlant media recipes are designed to track the formulation context, not to enforce exact measurements. Use them to record what went into a batch and attach the recipe to the stages that used it.

→Create a media recipe named by formulation and purpose — e.g. "MS 0.1 BAP — Multiplication" or "WPM 0.5 IBA — Rooting".
→Add ingredients with amounts and units. xPlant stores this as reference context, not a formulation calculator.
→When you prepare a batch, attach the recipe to the relevant stages. If you deviated (adjusted pH differently, swapped a salt source), note it in the stage transfer log.
→Review which recipes are used most often via the media recipe list — it helps identify which formulations to standardise first.

Common preparation issues

Agar won’t gel or gels unevenly

Likely cause: pH too low before autoclaving, or agar not fully suspended before dispensing.

Try: Target pH 5.8 before autoclaving. Stir agar thoroughly while hot. Check agar source — some suppliers have lot-to-lot quality variation.

Media turns brown after autoclaving

Likely cause: Over-autoclaving, temperature too high, or high sugar concentration.

Try: Check autoclave calibration. Reduce autoclave time for small volumes. Sucrose undergoes Maillard-type reactions at high heat — some browning is normal in small quantities.

Media contaminates within days

Likely cause: Loose vessel caps, handling before media cooled, or contaminated water source.

Try: Use autoclave-safe vented caps or foil. Handle vessels in laminar flow after autoclaving. Verify water source purity (use fresh distilled or 18 MΩ deionised).

Reference: MS basal medium (1 L)

Murashige and Skoog (1962) is the most widely used basal medium in tissue culture. The following table is a quick reference — use your lab's validated recipe or a quality premix where available.

Component	Amount	Note
Macro salts (MS premix)	4.4 g	Or weigh individual salts
Sucrose	30 g	Standard; reduce for some species
Myo-inositol	100 mg	Often included in premix
Thiamine HCl	0.1–1 mg	Often included in premix
Agar	7–8 g	Omit for liquid culture
Distilled water	To 1 L
pH	5.7–5.8	Adjust before autoclaving

Preparation steps

Gather materials

Analytical balance, distilled or deionised water, volumetric flask (1 L), magnetic stirrer + hotplate, pH meter, KOH or HCl for pH adjustment, agar (if solidifying), media salts and PGRs.

Dissolve salts

Add ~800 mL of distilled water to the flask. Weigh each macro- and micronutrient salt and dissolve in order of concentration (macros first). Stir gently; some salts may need gentle heat to dissolve fully.

Add sugar and vitamins

Add sucrose (typically 30 g/L for MS). Add vitamins (thiamine, glycine, myoinositol) if not included in a premix. Stir to dissolve.

Add plant growth regulators

Add PGRs (auxins, cytokinins) last before pH adjustment. Many PGRs are prepared as stock solutions (1000× or 10 000×) dissolved in KOH or ethanol — add the calculated volume from stock.

Adjust pH

Calibrate your pH meter. Adjust to pH 5.7–5.8 (or protocol-specific target) using 1 M KOH to raise or 1 M HCl to lower. pH will shift slightly on autoclaving — stop at 5.8 if autoclaving a solidified medium.

Add agar (solid media)

Bring volume to 1 L. Add agar (typically 7–8 g/L for standard solid media). Stir on hotplate until agar is fully suspended — it will not dissolve until autoclaved.

Dispense into vessels

Pour ~20–25 mL per culture tube or jar before autoclaving. Leave caps loose or use autoclave-safe vented caps. Do not overfill — agar expands slightly and needs headspace.

Autoclave

121 °C, 15 psi, 20 minutes (liquid cycle). Allow to cool to ~50–55 °C before pouring plates or adding heat-sensitive additives. Solidified media in vessels can cool in a rack.

Cool and store

Allow to solidify at room temperature. Inspect vessels for unusual colour, particulates, or contamination before use. Store at 4 °C for up to 4 weeks or at room temperature for up to 2 weeks (sealed, dark).

Logging batches in xPlant

xPlant media recipes are designed to track the formulation context, not to enforce exact measurements. Use them to record what went into a batch and attach the recipe to the stages that used it.

→Create a media recipe named by formulation and purpose — e.g. "MS 0.1 BAP — Multiplication" or "WPM 0.5 IBA — Rooting".

→Add ingredients with amounts and units. xPlant stores this as reference context, not a formulation calculator.

→When you prepare a batch, attach the recipe to the relevant stages. If you deviated (adjusted pH differently, swapped a salt source), note it in the stage transfer log.

→Review which recipes are used most often via the media recipe list — it helps identify which formulations to standardise first.

Common preparation issues

Agar won’t gel or gels unevenly

Likely cause: pH too low before autoclaving, or agar not fully suspended before dispensing.

Try: Target pH 5.8 before autoclaving. Stir agar thoroughly while hot. Check agar source — some suppliers have lot-to-lot quality variation.

Media turns brown after autoclaving

Likely cause: Over-autoclaving, temperature too high, or high sugar concentration.

Try: Check autoclave calibration. Reduce autoclave time for small volumes. Sucrose undergoes Maillard-type reactions at high heat — some browning is normal in small quantities.

Media contaminates within days

Likely cause: Loose vessel caps, handling before media cooled, or contaminated water source.

Try: Use autoclave-safe vented caps or foil. Handle vessels in laminar flow after autoclaving. Verify water source purity (use fresh distilled or 18 MΩ deionised).