R2A agar

R2A agar, a microbiological growth medium, is specifically formulated for the cultivation and enumeration of bacteria from potable water. It was developed by Reasoner and Geldreich in 1983, aiming to simulate the nutrient content of natural waters, which is typically lower than that found in more enriched laboratory media. This makes R2A agar particularly suitable for recovering slow-growing bacteria that inhabit aquatic environments and are often missed by conventional, richer media.

Composition[edit | edit source]

R2A agar's composition per liter of distilled water includes:

• 0.5 g of yeast extract,
• 0.5 g of proteose peptone,
• 0.5 g of casamino acids,
• 0.5 g of glucose,
• 0.5 g of starch,
• 0.3 g of dipotassium phosphate (K2HPO4),
• 0.05 g of magnesium sulfate (MgSO4),
• 0.3 g of sodium pyruvate,
• 15 g of agar,
• pH adjusted to 7.2.

Purpose and Usage[edit | edit source]

R2A agar is used in both research and practical applications, including the testing of drinking water and bottled water. Its low nutrient content slows down the growth rate of bacteria, allowing for the cultivation of typically overlooked slow-growing species. This property is particularly beneficial in environmental and public health contexts, where understanding the full scope of microbial populations in water sources is crucial.

Advantages[edit | edit source]

The primary advantage of R2A agar is its ability to mimic the nutrient levels of natural water, thereby providing a more accurate representation of water quality and potential health risks. It has been shown to recover a wider variety of bacteria, including those that are slow-growing or require lower nutrient levels for growth.

Limitations[edit | edit source]

While R2A agar is effective for isolating a diverse range of bacteria, it may not be suitable for detecting fast-growing, opportunistic pathogens that thrive in nutrient-rich environments. Additionally, the slow growth rate on R2A agar requires longer incubation times, typically around 7 days, which may not be ideal for rapid assessment needs.

Methodology[edit | edit source]

To use R2A agar for water testing, a sample of water is spread onto the surface of the agar plate and incubated at a temperature of 28°C for 7 days. After incubation, colonies are counted to estimate the number of viable bacteria present in the water sample. This method is aligned with guidelines provided by regulatory agencies for water quality testing.

Regulatory Aspects[edit | edit source]

R2A agar is recommended by various international standards and guidelines for the enumeration of heterotrophic bacteria in drinking water. Its use is supported by organizations such as the American Public Health Association (APHA), the American Water Works Association (AWWA), and the World Health Organization (WHO).

Conclusion[edit | edit source]

R2A agar represents a critical tool in environmental microbiology for assessing water quality and microbial diversity. Its formulation allows for the recovery and enumeration of a wide range of bacteria, including those that are slow-growing or have specific nutrient requirements, thereby providing a more comprehensive understanding of microbial populations in water sources.