Week 9 HW: Cell Free Systems

##Part 1 1.Advantages of Cell-Free Over In Vivo Expression Cell-free protein synthesis (CFPS) removes the cell as a “black box” and allows you directly control and observe every variable in real time: pH, redox potential, ionic strength, and cofactor concentration.

2.Main Components and Their Roles

Component	Role
Cell extract	Provides ribosomes, tRNA, synthetases, chaperones, and machinery
DNA/mRNA template	Encodes the target protein (plasmid or linear)
RNA polymerase	Transcribes DNA → mRNA (T7 RNAP is most common)
Amino acids	Raw building blocks for translation
Energy system	Supplies and recycles ATP/GTP to power translation
Salts and buffer	Maintains pH (~7.5) and ionic strength (Mg²⁺, K⁺ critical)
Additives	Chaperones, detergents, etc., added based on target needs

3.Energy Provision and ATP Regeneration

Translation is enormously ATP-hungry: every peptide bond costs ~4 high-energy phosphate bonds. In a tube, the initial ATP pool depletes within 30–60 minutes, stalling ribosomes and collapsing yield.

Phosphocreatine / Creatine Kinase System

ADP + phosphocreatine → ATP + creatine (catalyzed by creatine kinase)

Add phosphocreatine (~20 mM) and creatine kinase (~0.5 mg/mL).
Extends productive reaction time from ~1 hour to 3–6 hours.
Alternative: Maltose/maltodextrin system — a multi-enzyme cascade mimicking glycolysis, cheaper for large-scale reactions.

4.Prokaryotic vs. Eukaryotic Cell-Free Systems

Feature	Prokaryotic (E. coli)	Eukaryotic (wheat germ / CHO)
Post-translational mods	None	Glycosylation, phosphorylation, etc.
Cost	Low	High
Yield	High	Moderate
Best for	Simple cytosolic proteins	Mammalian proteins, antibodies, GPCRs

Prokaryotic Choice — T7 RNA Polymerase: Straightforward cytosolic protein, no PTMs needed, high yield required.
Eukaryotic Choice — Erythropoietin (EPO): Requires N-linked glycosylation for proper folding. A prokaryotic system would produce misfolded, inactive protein.

Designing Cell-Free Expression of a Membrane Protein

Membrane proteins are hydrophobic — without a lipid bilayer, they aggregate instantly.

Three Solubilization Strategies

Detergent micelles (DDM, digitonin) — Simplest; add directly to reaction.
Nanodiscs — Pre-assembled lipid bilayer discs; co-translate so protein inserts immediately.
Liposomes — Lipid vesicles that capture the protein as it emerges from the ribosome.

##Part 2 Synthetic Minimal Cell: Gut Microbiome Inflammation Sensor

1. Function

1a. What It Does — Input and Output

A liposome-based synthetic cell that detects elevated reactive oxygen species (ROS) in the gut lumen — a molecular signature of intestinal inflammation — and responds by producing and releasing butyrate, a short-chain fatty acid that suppresses NF-κB signaling and restores epithelial barrier integrity.

Feature	Description
Input	Hydrogen peroxide ($H_2O_2$) and superoxide — ROS elevated during gut inflammation (IBD, Crohn’s, colitis)
Output	Butyrate (butanoic acid) — anti-inflammatory metabolite that feeds colonocytes and suppresses immune activation

Analogy: Think of it like a smoke detector hardwired to a fire sprinkler — the same signal that trips the alarm also triggers the response, with no human intervention needed. The synthetic cell is silent in a healthy gut and active only when and where inflammation occurs.

1b. Could Cell-Free Tx/Tl Alone Do This Without Encapsulation?

No. There are three primary reasons:

Directionality: Without a membrane boundary, butyrate produced freely in solution would diffuse away immediately with no directional delivery to the epithelium.
Protection: The ROS-sensing gene circuit would be exposed to gut proteases and nucleases, degrading within minutes.
Threshold Control: There is no mechanism for threshold-gated release — the entire reaction would fire at once rather than responding proportionally to local ROS concentration.

1c. Could a Genetically Modified Natural Cell Do This?

Partially — but with serious limitations compared to a synthetic liposome:

Feature	Engineered Bacterium	Synthetic Liposome Cell
ROS sensing	Possible via OxyR regulon	Possible via OxyR-driven promoter
Butyrate synthesis	Yes — multiple chassis	Yes — encapsulated enzyme pathway
Immune clearance	High — triggers innate immunity	Minimal — PEGylated lipids are inert
Replication control	Requires auxotrophy kill switch	Non-replicating by design
Gene Transfer	Risk of horizontal transfer	Zero risk
Regulatory path	Extremely difficult (GMO in gut)	More tractable as a drug delivery device

1d. Desired Outcome

A synthetic cell administered orally (enteric-coated capsule) that survives transit to the colon, remains transcriptionally silent in healthy tissue, and activates butyrate synthesis specifically at inflamed foci where $H_2O_2$ exceeds threshold (~50 µM).

2. Component Design

2a. Membrane Composition

The membrane is designed to survive the harsh gut environment (low pH, bile salts) while remaining functional at 37°C.

Lipid	Role	Mol%
DPPC	High-Tm structural lipid; bile salt resistance	40%
POPE	Supports protein insertion; reduces curvature stress	25%
Cholesterol	Rigidifies bilayer; reduces permeability	25%
DSPE-PEG2000	PEG brush layer; prevents immune recognition	10%

2b. Encapsulated Contents

The “cytoplasm” of the synthetic cell contains the following:

Tx/Tl Machinery: E. coli cell-free extract (ribosomes, tRNA, chaperones), T7 RNA Polymerase, and the OxyR-responsive promoter plasmid.
Pre-loaded Enzymes: Acetyl-CoA acetyltransferase (ThlA) for fast initial response.
Small Molecules: Acetyl-CoA (2 mM), Phosphocreatine (20 mM) + creatine kinase (0.5 mg/mL), all 20 amino acids (5 mM each), and essential cofactors (NAD⁺/NADH, CoA).

2c. Tx/Tl System Origin: Bacterial (E. coli)

A prokaryotic system is preferred because the OxyR transcription factor and the butyrate synthesis enzymes (from Clostridium) are natively bacterial. No complex post-translational modifications (PTMs) are required, making the high-yield E. coli extract the most efficient choice.

2d. Communication with the Environment

Sensing (IN — Passive): $H_2O_2$ crosses lipid bilayers freely via passive diffusion. Inside, it oxidizes OxyR, switching it from a repressor to an activator.
Secretion (OUT — Active): We express VDAC-1 (voltage-dependent anion channel 1). While butyrate is anionic at physiological pH, the expressed VDAC-1 pores permit rapid efflux.

3. Experimental Details

3a. Complete Genes and Lipids

Gene	Organism	Role
oxyR	E. coli K-12	ROS-activated transcription factor
thlA	C. acetobutylicum	Step 1: 2 acetyl-CoA → acetoacetyl-CoA
hbd	C. acetobutylicum	Step 2: → 3-hydroxybutyryl-CoA
crt	C. acetobutylicum	Step 3: → crotonyl-CoA
bcd/etfAB	C. acetobutylicum	Step 4: → butyryl-CoA
ptb/buk	C. acetobutylicum	Steps 5–6: → butyrate
VDAC1	H. sapiens	Membrane pore for butyrate efflux

3b. Measuring System Function

Validation is performed through a tiered strategy:

Tier 1: ROS-responsive expression: Use a GFP reporter to confirm the OxyR circuit activates at the ~50 µM $H_2O_2$ threshold.
Tier 2: Butyrate synthesis: Quantify butyrate production in bulk extract using GC-MS or enzymatic assays.
Tier 3: Pore function: Use ANTS/DPX dye efflux assays to confirm VDAC-1 correctly inserts into the liposome membrane.
Tier 4: Integrated function: Measure butyrate secretion from encapsulated cells in simulated healthy (5 µM $H_2O_2$) vs. inflamed (100 µM $H_2O_2$) conditions.
Tier 5: Bioactivity: Apply the output to Caco-2 cells and measure the reduction in inflammatory markers (IL-8/NF-κB).

##Part 3. Aura-Weave (Smart Medical Wearables)

1. One-Sentence Summary Pitch

Aura-Weave is a smart, disposable textile liner for adult incontinence garments that uses freeze-dried cell-free extracts to seamlessly detect and visually report urinary tract infections (UTIs) by changing color when exposed to infected urine.

2. How the Idea Works in Detail

The Aura-Weave liner features a middle diagnostic layer composed of a highly absorbent cellulose matrix (similar to filter paper). This matrix is pre-loaded with a lyophilized (freeze-dried) cell-free extract (CFE), specific engineered DNA circuits, and pH buffers.

The Mechanism:

Dormancy: The system remains completely inactive on the shelf in its dry state.
Activation: When the wearer voids urine, the warm liquid acts as the natural rehydration trigger, “booting up” the biological transcription and translation machinery.
Detection: If specific UTI biomarkers are present—such as nitrites, leukocyte esterase, or bacterial quorum-sensing molecules—the genetic circuit is triggered.
Visual Output: The circuit drives the rapid expression of a vibrant chromoprotein (like AmilCP). Within 45 to 60 minutes, a clear blue warning symbol permeates to the outer visible edge of the textile.

Visual Indicator: A blue symbol or color change alerts the caregiver immediately without requiring a manual diagnostic test.

3. Societal Challenge and Market Need

This addresses the “silent crisis” of UTIs in elderly, bedridden, and cognitively impaired populations (such as those with Alzheimer’s or dementia).

Communication Barriers: These patients often cannot communicate early symptoms like pain or urgency, leading to delayed diagnosis.
Medical Risks: Late-stage UTIs frequently progress to severe kidney infections, sepsis, and costly hospitalizations.
Non-Invasive Monitoring: Aura-Weave eliminates the difficult, messy, and stress-inducing process of collecting a clean urine sample from an uncooperative patient, allowing for continuous, passive health monitoring in nursing homes and home-care settings.

4. Addressing Cell-Free Limitations

Limitation	Aura-Weave Strategy
Water Activation	The Built-in Trigger: In this context, rehydration is a feature. The CFE stays inactive until the exact moment the patient urinates, ensuring the test only runs when a sample is provided.
Stability	Sugar Matrix Stabilization: To ensure a shelf life of over a year, the CFE and DNA are co-lyophilized with a stabilizing sugar (trehalose) and a strong buffer (HEPES), locking proteins in a stable, glass-like state at room temperature.
One-Time Use	Lifecycle Alignment: Incontinence liners are inherently single-use. The biological sensor’s lifecycle perfectly matches the textile’s lifecycle; once soiled and read, the garment is safely discarded.

Technical Specifications

Target Biomarkers: Nitrites, Leukocyte Esterase, Quorum-Sensing molecules.
Reporter Protein: AmilCP (Chromoprotein).
Time to Result: 45–60 minutes post-activation.
Storage Requirements: Room temperature (stabilized via Trehalose).

##Part 4

The Challenge: Current missions detect “bricks” (organic molecules) but not “factories” (active life).
Strategy: Use FD-CF systems to detect ATP Synthesis and 16S rRNA genes.
Reasoning: Only active biology synthesizes ATP; abiotic chemistry (like meteorites) might have organics but no coordinated metabolism.
Experimental Plan: Compare Mars simulant spiked with extremophiles against sterile simulant and abiotic meteorite extracts.