Quick answer
How much UV-C an organism needs has surprisingly little to do with how "tough" it seems against chemicals. UV resistance is driven by biology, mainly two things:
- Genome type and repair — what the genetic material is, and whether it can be repaired after UV damage.
- Physical shielding — spore coats, cyst walls and pigments that keep UV from the genome in the first place.
The headline example is a complete reversal: Cryptosporidium laughs off chlorine (a notorious drinking-water problem) yet falls to a tiny UV dose. So the right question is never "is this germ tough?" but "what is its UV biology?" — which is exactly what sets the dose you must design for.
1. The master variable: genome structure and host repair
UV-C inactivates by damaging nucleic acid (forming dimers that block replication). Whether that damage sticks depends on the genome:
- Double-stranded DNA viruses — repairable, therefore resistant. Adenovirus is the classic case: its dsDNA genome looks like the host cell's own DNA, so once inside a cell the host's DNA-repair machinery (transcription-coupled nucleotide-excision repair) fixes the UV lesions. The effect is dose-dependent — studies show doses ≤15 mJ/cm² produce lesions without loss of infectivity, while ≥20 mJ/cm² are needed for significant (>1-log) inactivation.
- Single-stranded RNA/DNA viruses — not host-repairable, therefore sensitive. A single-stranded or RNA genome is not recognised by host DNA-repair pathways, so the damage is not undone and these viruses are inherently easier to inactivate.
(A molecular nuance: RNA actually forms UV lesions less readily than DNA in the first place — UV photochemistry is strongly sequence- and conformation-dependent. But in practice the repair factor usually dominates an organism's effective resistance.)
2. The resistance ladder — and its caveats
Roughly, from easiest to hardest to inactivate with UV-C (always organism-specific — see the dose anchors):
| Class | Relative UV resistance | Why |
|---|---|---|
| Vegetative bacteria | low (easy) | exposed genome, limited shielding |
| ss-genome viruses | low–moderate | damage not host-repaired |
| Fungi (Candida, Aspergillus) | moderate | larger, pigmented, multilayer wall, eukaryotic repair |
| dsDNA viruses (adenovirus) | high | host DNA-repair rescues the genome |
| Bacterial spores | very high | SASP + dehydration (Section 3) |
A concrete contrast: 99.9% inactivation of vegetative bacteria (e.g. P. aeruginosa) is reached in seconds, whereas fungi such as Candida albicans and Aspergillus fumigatus need several times longer under the same lamp.
3. Bacterial spores — the champions, and why
Endospores (Bacillus, Clostridioides difficile) are the most UV-tolerant common targets, by a specific, well-understood mechanism:
- Small acid-soluble proteins (SASP). α/β-type SASP — making up roughly 20% of spore protein and conserved across all endospore-formers — bind the spore's DNA and force it into an A-form conformation. In that geometry UV produces a different, more repairable lesion (the "spore photoproduct") instead of the usual thymine dimers, and that lesion is efficiently fixed when the spore germinates. Spores engineered without SASP are dramatically more UV-sensitive.
- Low core water content adds further resistance to environmentally relevant UV.
This is why spore-formers (e.g. C. difficile in healthcare) are the design worst-case: size your dose for the spore, and everything easier is covered.
4. The protozoan reversal — chlorine-proof, UV-vulnerable
Here the intuition breaks completely, and it is the single most important practical fact in this article:
- Cryptosporidium and Giardia have thick, robust (oo)cyst walls that make them highly resistant to chlorine — historically a serious failure mode for chemical drinking-water treatment.
- Yet they are very sensitive to UV: a low UV dose blocks their ability to replicate/infect, even though it doesn't visibly "destroy" the organism.
This reversal is precisely why UV won a place in drinking-water treatment — and why regulators grant validated UV reactors a Cryptosporidium/Giardia inactivation credit (see validation).
The honest nuance: UV's effectiveness here is measured by infectivity, not crude "viability". An oocyst can remain structurally intact and even excyst, yet be unable to cause infection because its genome can no longer be replicated. Studies that measure raw viability (e.g. ~230 mJ/cm² for 2-log by an excystation assay) report far higher "doses" than infectivity-based inactivation (orders of magnitude lower). For UV, infectivity is the meaningful endpoint — but be alert to which assay a claim is based on.
5. Repair is the thread through all of it
Notice the recurring theme: adenovirus (host repair), bacteria (a whole "UV-resistome" of sense/shield/detoxify/repair/tolerate functions, taken to extremes in Deinococcus), and the photoreactivation/dark-repair covered in the dose article. Repair capacity is often what separates a resistant organism from a sensitive one — which is why real designs carry a dose margin above the bare lab D-value and why downstream conditions matter.
6. Practical: design for your worst-case organism
- Identify the most resistant relevant target — its biology (genome, spore coat, repair) sets the required dose, not a generic "kills 99.9% of bacteria" claim.
- Match the validation surrogate — this is why biodosimetry uses defined surrogates (MS2, T1): the validated RED depends on the test organism's UV sensitivity.
- Never extrapolate across classes — a dose that clears vegetative bacteria may do almost nothing to a spore or an adenovirus.
Cross-references
- UV-C Dose & Log Reduction — /knowledge/uv-c-dose-and-log-reduction: the dose-per-log anchors this article explains.
- UV-C Validation & Dose Measurement — /knowledge/uv-c-validation-and-dose-measurement: why surrogate choice matters; the Crypto/Giardia credit.
- Air vs. Surface vs. Water — /knowledge/uv-c-air-surface-water-in-practice: where these organisms actually live.
Sources
- Setlow et al. — Essential role of SASP in resistance of B. subtilis spores to UV (J. Bacteriol., PMC) — SASP/A-form/spore photoproduct.
- Roles of SASP and core water content in B. subtilis spore UV survival (AEM) — SASP + dehydration, ~20% spore protein.
- SASP of Clostridioides difficile are important for UV resistance (PLOS Pathogens) — spore-former worst-case.
- UV Disinfection of Adenoviruses: molecular DNA-damage efficiency (AEM) — dsDNA + host repair.
- Adenovirus dose-dependent repair & delayed host DNA-damage response (ES&T) — ≤15 / ≥20 mJ/cm² thresholds.
- RNA is more UV resistant than DNA — lesion formation is sequence/conformation dependent (ResearchGate) — genome-chemistry nuance.
- Efficiency of chlorine and UV in inactivation of Cryptosporidium and Giardia (PLOS One / PMC) — chlorine-resistant, UV-sensitive.
- Efficacy of UV irradiation in inactivating Cryptosporidium parvum oocysts (PMC) — infectivity vs. viability endpoint.